#METABOLOMICS WORKBENCH ptth222_20180124_070246_mwtab.txt DATATRACK_ID:1304 STUDY_ID:ST000927 ANALYSIS_ID:AN001520 PROJECT_ID:PR000642
VERSION             	1
CREATED_ON             	January 24, 2018, 6:41 pm
#PROJECT
PR:PROJECT_TITLE                 	Breast Cancer Metabolism
PR:PROJECT_SUMMARY               	The program comprises three project areas utilizing stable isotope resolved
PR:PROJECT_SUMMARY               	metabolomics to gain a mechanistic understanding of NSCLC in situ. The projects
PR:PROJECT_SUMMARY               	combine cell culture, animal models and human subjects to define the influence
PR:PROJECT_SUMMARY               	of the tumor microenvironment on cancer progression.
PR:INSTITUTE                     	University of Kentucky
PR:LAST_NAME                     	Lane
PR:FIRST_NAME                    	Andrew
PR:ADDRESS                       	Rm 516 Biopharm Complex, 789 S. Limestone St.,Univ. of Kentucky, Lexington, KY
PR:ADDRESS                       	40536
PR:EMAIL                         	andrewlane@gmail.com
PR:PHONE                         	8592182868
#STUDY
ST:STUDY_TITLE                   	Probing the metabolic phenotype of breast cancer cells by multiple tracer stable
ST:STUDY_TITLE                   	isotope resolved metabolomics (part II)
ST:STUDY_SUMMARY                 	Breast cancers vary by their origin and specific set of genetic lesions, which
ST:STUDY_SUMMARY                 	gives rise to distinct phenotypes and differential response to targeted and
ST:STUDY_SUMMARY                 	untargeted chemotherapies. To explore the functional differences of different
ST:STUDY_SUMMARY                 	breast cell types, we performed Stable Isotope Resolved Metabolomics (SIRM)
ST:STUDY_SUMMARY                 	studies of one primary breast (HMEC) and three breast cancer cells (MCF-7,
ST:STUDY_SUMMARY                 	MDAMB-231, and ZR75-1) having distinct genotypes and growth characteristics,
ST:STUDY_SUMMARY                 	using 13C6-glucose, 13C-1+2-glucose, 13C5,15N2-Gln, 13C3-glycerol, and
ST:STUDY_SUMMARY                 	13C8-octanoate as tracers. These tracers were designed to probe the central
ST:STUDY_SUMMARY                 	energy producing and anabolic pathways (glycolysis, pentose phosphate pathway,
ST:STUDY_SUMMARY                 	Krebs Cycle, glutaminolysis, nucleotide synthesis and lipid turnover). We found
ST:STUDY_SUMMARY                 	that glycolysis was not associated with the rate of breast cancer cell
ST:STUDY_SUMMARY                 	proliferation, glutaminolysis did not support lipid synthesis in primary breast
ST:STUDY_SUMMARY                 	or breast cancer cells, but was a major contributor to pyrimidine ring synthesis
ST:STUDY_SUMMARY                 	in all cell types; anaplerotic pyruvate carboxylation was activated in breast
ST:STUDY_SUMMARY                 	cancer versus primary cells. We also found that glucose metabolism in individual
ST:STUDY_SUMMARY                 	breast cancer cell lines differed between in vitro cultures and tumor
ST:STUDY_SUMMARY                 	xenografts, but not the metabolic distinctions between cell lines, which may
ST:STUDY_SUMMARY                 	reflect the influence of tumor architecture/microenvironment.
ST:INSTITUTE                     	University of Kentucky
ST:LAST_NAME                     	Lane
ST:FIRST_NAME                    	Andrew
ST:ADDRESS                       	Rm 516 Biopharm Complex, 789 S. Limestone St.,Univ. of Kentucky, Lexington, KY
ST:ADDRESS                       	40536
ST:EMAIL                         	andrewlane@gmail.com
ST:PHONE                         	8592182868
#SUBJECT
SU:SUBJECT_TYPE                  	Human
SU:SUBJECT_SPECIES               	Homo sapiens
SU:TAXONOMY_ID                   	9606
#SUBJECT_SAMPLE_FACTORS:         	SUBJECT(optional)[tab]SAMPLE[tab]FACTORS(NAME:VALUE pairs separated by |)[tab]Additional sample data
SUBJECT_SAMPLE_FACTORS           	-	HMEC_UC13Glc_Ctl_toc50	Cell Line:HMEC | Tracer:Uniformly Labelled Glucose	Tracer_Abbreviated=U-C13-Glc; Cancer=Not Cancer
SUBJECT_SAMPLE_FACTORS           	-	MCF7_UC13Glc_Ctl_toc50	Cell Line:MCF-7 | Tracer:Uniformly Labelled Glucose	Tracer_Abbreviated=U-C13-Glc; Cancer=Cancer
SUBJECT_SAMPLE_FACTORS           	-	ZR75_1_cells_24h_c13glcSep09_toc50	Cell Line:ZR-75-1 | Tracer:Uniformly Labelled Glucose	Tracer_Abbreviated=U-C13-Glc; Cancer=Cancer
SUBJECT_SAMPLE_FACTORS           	-	HMEC_C13Gln_Ctl_toc50	Cell Line:HMEC | Tracer:Uniformly Labelled Glutamine	Tracer_Abbreviated=U-C13_N15-Gln; Cancer=Not Cancer
SUBJECT_SAMPLE_FACTORS           	-	MCF7_C13Gln_Ctl_toc50	Cell Line:MCF-7 | Tracer:Uniformly Labelled Glutamine	Tracer_Abbreviated=U-C13_N15-Gln; Cancer=Cancer
SUBJECT_SAMPLE_FACTORS           	-	ZR751_Nor_HiGlc_U13C15NGln_TOCSY	Cell Line:ZR-75-1 | Tracer:Uniformly Labelled Glutamine	Tracer_Abbreviated=U-C13_N15-Gln; Cancer=Cancer
#COLLECTION
CO:COLLECTION_SUMMARY            	Cells were cultured in various media then harvested after 24 hours.
CO:SAMPLE_TYPE                   	Cells
#TREATMENT
TR:TREATMENT_SUMMARY             	None
#SAMPLEPREP
SP:SAMPLEPREP_SUMMARY            	Cell lines are seperated into polar, non-polar, protein, and media.
#CHROMATOGRAPHY
CH:CHROMATOGRAPHY_TYPE           	-
CH:INSTRUMENT_NAME               	-
CH:COLUMN_NAME                   	-
#ANALYSIS
AN:ANALYSIS_TYPE                 	NMR
#NMR
NM:INSTRUMENT_NAME               	INOVA
NM:INSTRUMENT_TYPE               	CW-NMR
NM:NMR_EXPERIMENT_TYPE           	Other
NM:SPECTROMETER_FREQUENCY        	800 MHz
#NMR_METABOLITE_DATA
NMR_METABOLITE_DATA:UNITS        	area
NMR_METABOLITE_DATA_START
Samples	HMEC_C13Gln_Ctl_toc50	HMEC_UC13Glc_Ctl_toc50	MCF7_C13Gln_Ctl_toc50	MCF7_UC13Glc_Ctl_toc50	ZR75_1_cells_24h_c13glcSep09_toc50	ZR751_Nor_HiGlc_U13C15NGln_TOCSY
Factors	Cell Line:HMEC | Tracer:Uniformly Labelled Glutamine	Cell Line:HMEC | Tracer:Uniformly Labelled Glucose	Cell Line:MCF-7 | Tracer:Uniformly Labelled Glutamine	Cell Line:MCF-7 | Tracer:Uniformly Labelled Glucose	Cell Line:ZR-75-1 | Tracer:Uniformly Labelled Glucose	Cell Line:ZR-75-1 | Tracer:Uniformly Labelled Glutamine
UXP-5 13C-A	50.74038416	57.01434766	315.6179647	415.98389	318.7578252	157.6554549
UXP-5 13C-B	86.42896764	157.3195258	340.7416454	404.7737169	225.5226737	425.8632207
UXP-5,6 13C-A	500.507461	103.9207387	922.8158171	627.2578756	1415.874749	622.1238667
UXP-5,6 13C-B	538.2189425	89.07780904	867.864989	447.1612448	1107.10075	1303.257013
UXP-6	456.3852955	1082.995872	2721.184463	2194.277233	3932.602853	617.0999188
UXP-6 13C-A	82.42272487	80.22959021	402.6092283	690.9317071	347.3962358	267.7202832
UXP-6 13C-B	238.1921457	111.4472882	435.3887976	508.4034492	332.1889378	150.29
NMR_METABOLITE_DATA_END
#METABOLITES
METABOLITES_START
metabolite_name	retention index	quantified m/z	PubChem ID	KEGG ID	Common Name	Hydrogen Number	Isotope	PPM Range (1)	PPM Range (2)
UXP-5 13C-A					Uridine Phosphates	5	13C	7.93186439797907 - 7.967447801	5.79290009505425 - 5.834791062
UXP-5 13C-B					Uridine Phosphates	5	13C	7.93610290815661 - 7.972723056	6.08994864749875 - 6.10982575
UXP-5,6 13C-A					Uridine Phosphates	5	13C	7.77607998762907 - 8.106954655	5.78768499084674 - 6.110864608
UXP-5,6 13C-B					Uridine Phosphates	5	13C	7.77890697522207 - 8.111280041	5.80200553239918 - 6.115338917
UXP-6					Uridine Phosphates	6	13C	7.93377342544742 - 7.983361653	5.942904357 - 5.96340861810778
UXP-6 13C-A					Uridine Phosphates	6	13C	7.77851358447656 - 8.101883111	5.94440660086254 - 6.106839021
UXP-6 13C-B					Uridine Phosphates	6	13C	8.08405619244877 - 8.111280042	5.94501676112817 - 5.967740509
METABOLITES_END
#END