#METABOLOMICS WORKBENCH STUDY_ID:ST000185 ANALYSIS_ID:AN000284 PROJECT_ID:PR000158
VERSION             	1
CREATED_ON          	01-15-2019
#PROJECT
PR:PROJECT_TITLE                 	LEC metabolomics
PR:PROJECT_SUMMARY               	Comparison of metabolomic profile in LECs derived from normal and shunt animals
PR:INSTITUTE                     	University of California, San Francisco
PR:DEPARTMENT                    	Pediatrics
PR:LABORATORY                    	Fineman Lab
PR:LAST_NAME                     	Fineman
PR:FIRST_NAME                    	Jeffrey
PR:ADDRESS                       	San Francisco, CA
PR:EMAIL                         	jeff.fineman@ucsf.edu
PR:PHONE                         	415-502-6390
PR:DOI                           	http://dx.doi.org/10.21228/M8T01Q
#STUDY
ST:STUDY_TITLE                   	Fetal Lambs vascular graft Normal v Shunt LECs
ST:STUDY_TYPE                    	Glycolysis/TCA/Nucleotide analysis (tissue/cells)
ST:STUDY_SUMMARY                 	We recently reported superior right ventricle (RV) performance in response to
ST:STUDY_SUMMARY                 	acute afterload challenge in lambs with a model of congenital heart disease with
ST:STUDY_SUMMARY                 	chronic left-to-right cardiac shunts. Compared with control animals, shunt lambs
ST:STUDY_SUMMARY                 	demonstrated increased contractility because of an enhanced Anrep effect (the
ST:STUDY_SUMMARY                 	slow increase in contractility following myocyte stretch). This advantageous
ST:STUDY_SUMMARY                 	physiological response may reflect preservation of a fetal phenotype, since the
ST:STUDY_SUMMARY                 	RV of shunt lambs remains exposed to increased pressure postnatally. Nitric
ST:STUDY_SUMMARY                 	oxide (NO) production by NO synthase (NOS) is activated by myocyte stretch and
ST:STUDY_SUMMARY                 	is a necessary intermediary of the Anrep response. The purpose of this study was
ST:STUDY_SUMMARY                 	to test the hypothesis that NO signaling is increased in the RV of fetal lambs
ST:STUDY_SUMMARY                 	compared with controls and shunt lambs have persistence of this fetal pattern.
ST:STUDY_SUMMARY                 	An 8-mm graft was placed between the pulmonary artery and aorta in fetal lambs
ST:STUDY_SUMMARY                 	(shunt). NOS isoform expression, activity, and association with activating
ST:STUDY_SUMMARY                 	cofactors were determined in fetal tissue obtained during late-gestation and in
ST:STUDY_SUMMARY                 	4-wk-old juvenile shunt and control lambs. We demonstrated increased RNA and
ST:STUDY_SUMMARY                 	protein expression of NOS isoforms and increased total NOS activity in the RV of
ST:STUDY_SUMMARY                 	both shunt and fetal lambs compared with control. We also found increased NOS
ST:STUDY_SUMMARY                 	activation and association with cofactors in shunt and fetal RV compared with
ST:STUDY_SUMMARY                 	control. These data demonstrate preserved fetal NOS phenotype and NO signaling
ST:STUDY_SUMMARY                 	in shunt RV, which may partially explain the mechanism underlying the adaptive
ST:STUDY_SUMMARY                 	response to increased afterload seen in the RV of shunt lambs. Research is
ST:STUDY_SUMMARY                 	published, core data not used but project description is relevant:
ST:STUDY_SUMMARY                 	http://ajpheart.physiology.org/content/309/1/H157.long
ST:INSTITUTE                     	University of Michigan
ST:DEPARTMENT                    	Biomedical Research Core Facilities
ST:LABORATORY                    	Metabolomics core
ST:LAST_NAME                     	Kachman
ST:FIRST_NAME                    	Maureen
ST:ADDRESS                       	6300 Brehm Tower, 1000 Wall Street, Ann Arbor, MI 48105-5714
ST:EMAIL                         	mkachman@umich.edu
ST:PHONE                         	-
#SUBJECT
SU:SUBJECT_TYPE                  	Animal
SU:SUBJECT_SPECIES               	Ovis aries
SU:TAXONOMY_ID                   	9940
SU:SPECIES_GROUP                 	Mammal
#SUBJECT_SAMPLE_FACTORS:         	SUBJECT(optional)[tab]SAMPLE[tab]FACTORS(NAME:VALUE pairs separated by |)[tab]Additional sample data
SUBJECT_SAMPLE_FACTORS           	SU0011546	S00017020	Type:increased flow	
SUBJECT_SAMPLE_FACTORS           	SU0011547	S00017021	Type:increased flow	
SUBJECT_SAMPLE_FACTORS           	SU0011548	S00017022	Type:increased flow	
SUBJECT_SAMPLE_FACTORS           	SU0011543	S00017017	Type:normal control	
SUBJECT_SAMPLE_FACTORS           	SU0011544	S00017018	Type:normal control	
SUBJECT_SAMPLE_FACTORS           	SU0011545	S00017019	Type:normal control	
#COLLECTION
CO:SAMPLE_TYPE                   	Endothelial Cells
CO:COLLECTION_SUMMARY            	-
#TREATMENT
TR:TREATMENT_SUMMARY             	-
#SAMPLEPREP
SP:SAMPLEPREP_PROTOCOL_FILENAME  	Gly-TCA-nucleotides_analysis_protocol-2015-03-09.docx
SP:SAMPLEPREP_SUMMARY            	-
#CHROMATOGRAPHY
CH:METHODS_ID                    	AQM020
CH:METHODS_FILENAME              	QTOF-002-HILIC-35min-1mm-No_Insert.m.zip
CH:INSTRUMENT_NAME               	Agilent 1260
CH:COLUMN_NAME                   	Phenomenex Luna NH2 (150 x 1mm, 3um)
CH:CHROMATOGRAPHY_TYPE           	HILIC
#ANALYSIS
AN:LABORATORY_NAME               	MRC2 (University of Michigan)
AN:ANALYSIS_TYPE                 	MS
AN:ACQUISITION_PARAMETERS_FILE   	QTOF-002-HILIC-35min-1mm-No_Insert.m.zip
#MS
MS:MS_COMMENTS                   	-
MS:INSTRUMENT_NAME               	Agilent 6530 QTOF
MS:INSTRUMENT_TYPE               	QTOF
MS:MS_TYPE                       	ESI
MS:ION_MODE                      	NEGATIVE
#MS_METABOLITE_DATA
MS_METABOLITE_DATA:UNITS         	pmol/µg protein
MS_METABOLITE_DATA_START
Samples	S00017020	S00017021	S00017022	S00017017	S00017018	S00017019
Factors	Type:increased flow	Type:increased flow	Type:increased flow	Type:normal control	Type:normal control	Type:normal control	
2 or 3-phosphoglycerate_2PG/3PG	0.8978	0.3447	0.2680	6.4525	2.9002	6.3058
6-Phosphogluconate	0.6816	0.5188	0.3125	1.9113	1.4771	3.7586
Acetyl-CoA	0.1221			0.7683	0.5710	0.8624
ADP	21.4299	16.3787	15.1622	67.1431	40.6175	51.8677
AMP	9.3438	7.0078	7.4143	178.2130	68.4896	122.5572
ATP	66.8491	45.4450	39.1587	81.5229	90.1356	68.5431
Citrate or Isocitrate	30.3007	77.3516	33.7218	208.7459	129.0972	71.8109
flavin adenine dinucleotide	0.0975	0.1405	0.1166	0.3954	0.2555	0.3425
Fructose 1_6-bisphosphate	3.4687	1.1181	1.1003	16.3895	9.1119	15.0493
Glucose 6-phosphate or fructose-6-phosphate	16.2806	11.1167	7.8941	137.8086	33.0055	107.1428
Malate	42.5975	95.4928	36.2395	44.2528	36.1339	
nicotinamide adenine dinucleotide phosphate oxidized	1.2664	1.1893	1.0154	3.6640	2.3189	3.4695
Phosphoenolpyruvate	1.7034	3.3100	0.9094	6.3348	7.7797	4.6110
Ribose-5-phosphate or xylulose 5-phosphate	4.0956	1.1797	1.5413	11.6761	4.3669	8.9582
MS_METABOLITE_DATA_END
#METABOLITES
METABOLITES_START
metabolite_name	pubchem_id	inchi_key	kegg_id	other_id	other_id_type	ri	ri_type	moverz_quant	
2 or 3-phosphoglycerate_2PG/3PG	724		C00597	2PG/3PG	UM_Target_ID				
6-Phosphogluconate	91493		C00345	6PG	UM_Target_ID				
Acetyl-CoA	444493		C00024	aCoA	UM_Target_ID				
ADP	6022		C00008	ADP	UM_Target_ID				
AMP	6083		C00020	AMP	UM_Target_ID				
ATP	5957		C00002	ATP	UM_Target_ID				
Citrate or Isocitrate	311		C00158	CIT/ICIT	UM_Target_ID				
flavin adenine dinucleotide	643975		C00016	FAD	UM_Target_ID				
Fructose 1,6-bisphosphate	172313		C00354	FBP	UM_Target_ID				
Glucose 6-phosphate or fructose-6-phosphate	5958		C00092	G6P/F6P	UM_Target_ID				
Malate	222656		C00149	MAL	UM_Target_ID				
nicotinamide adenine dinucleotide phosphate oxidized	5886		C00006	NADP	UM_Target_ID				
Phosphoenolpyruvate	1005		C00074	PEP	UM_Target_ID				
Ribose-5-phosphate or xylulose 5-phosphate	77982		C00117	R5P/X5P	UM_Target_ID				
METABOLITES_END
#END