Summary of Study ST002529

This data is available at the NIH Common Fund's National Metabolomics Data Repository (NMDR) website, the Metabolomics Workbench, https://www.metabolomicsworkbench.org, where it has been assigned Project ID PR001627. The data can be accessed directly via it's Project DOI: 10.21228/M8D434 This work is supported by NIH grant, U2C- DK119886.

See: https://www.metabolomicsworkbench.org/about/howtocite.php

This study contains a large results data set and is not available in the mwTab file. It is only available for download via FTP as data file(s) here.

Study ID	ST002529
Study Title	In vivo 15N2-glutamine tracing by jugular vein infusion in PDAC-tumor bearing Lyz2-Arg1 and control mice
Study Summary	We assessed the relative levels of urea cycle related metabolites in PDAC tumors in Lyz2-Cre+/+; Arg1fl/fl compared to Arg1fl/fl control host animals.
Institute	University of Chicago
Last Name	Apiz Saab
First Name	Juan
Address	929 E. 57th St.
Email	japizsaab@uchicago.edu
Phone	7738346506
Submit Date	2023-03-24
Raw Data Available	Yes
Raw Data File Type(s)	mzML
Analysis Type Detail	LC-MS
Release Date	2023-04-13
Release Version	1

Select appropriate tab below to view additional metadata details:

Project:

Project ID:	PR001627
Project DOI:	doi: 10.21228/M8D434
Project Title:	Pancreatic tumors activate arginine biosynthesis to adapt to myeloid-driven amino acid stress
Project Summary:	Nutrient stress in the tumor microenvironment requires cancer cells to adopt adaptive metabolic programs to maintain survival and proliferation. Therefore, knowledge of microenvironmental nutrient levels and how cancer cells cope with such nutrition is critical to understand the metabolism underpinning cancer cell biology. Previously, we performed quantitative metabolomics of the interstitial fluid (the local perfusate) of murine pancreatic ductal adenocarcinoma (PDAC) tumors to comprehensively characterize nutrient availability in the microenvironment of these tumors (Sullivan et al., 2019a). Here, we develop Tumor Interstitial Fluid Medium (TIFM), a cell culture medium that contains nutrient levels representative of the PDAC microenvironment, enabling study of PDAC metabolism under physiological nutrition. We show that PDAC cells cultured in TIFM, compared to standard laboratory models, adopt a cellular state more similar to PDAC cells in tumors. Further, using the TIFM model we identified arginine biosynthesis as a metabolic adaptation PDAC cells engage to cope with microenvironmental arginine starvation driven by myeloid cells in PDAC tumors. Altogether, these data show that nutrient availability in tumors is an important determinant of cancer cell metabolism and behavior, and cell culture models that incorporate physiological nutrient availability have improved fidelity and enable the discovery of novel cancer metabolic phenotypes.
Institute:	University of Chicago
Last Name:	Apiz Saab
First Name:	Juan
Address:	929 E. 57th St.
Email:	japizsaab@uchicago.edu
Phone:	7738346506

Subject:

Subject ID:	SU002629
Subject Type:	Mammal
Subject Species:	Mus musculus
Taxonomy ID:	10090

Factors:

Subject type: Mammal; Subject species: Mus musculus (Factor headings shown in green)

mb_sample_id	local_sample_id	Sample type	Condition
SA254631	A35097-120	Plasma	Arg1fl/fl
SA254632	A35097-0	Plasma	Arg1fl/fl
SA254633	A35096-120	Plasma	Arg1fl/fl
SA254634	A35097-240	Plasma	Arg1fl/fl
SA254635	A35096-240	Plasma	Arg1fl/fl
SA254636	A35098-0	Plasma	Arg1fl/fl
SA254637	A35098-30	Plasma	Arg1fl/fl
SA254638	A35098-240	Plasma	Arg1fl/fl
SA254639	A35098-120	Plasma	Arg1fl/fl
SA254640	A35096-0	Plasma	Arg1fl/fl
SA254641	A35097-30	Plasma	Arg1fl/fl
SA254642	A35096-30	Plasma	Arg1fl/fl
SA254643	0789-120	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254644	0785-240	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254645	A35465-0	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254646	0787-0	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254647	0787-120	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254648	0787-30	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254649	0787-240	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254650	A35465-120	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254651	A35465-240	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254652	A35469-30	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254653	0785-120	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254654	A35469-240	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254655	A35469-120	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254656	A35465-30	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254657	A35469-0	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254658	0788-0	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254659	0785-30	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254660	A35066-240	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254661	A35066-30	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254662	A35066-120	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254663	0788-120	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254664	0789-240	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254665	0789-30	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254666	A35089-0	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254667	A35066-0	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254668	0788-240	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254669	A35089-120	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254670	0788-30	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254671	0785-0	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254672	0789-0	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254673	A35089-240	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254674	A35089-30	Plasma	Lyz2-Cre+/+; Arg1fl/fl
SA254675	A35098_tumor_Control	Tumor	Arg1fl/fl
SA254676	A35097_tumor_Control	Tumor	Arg1fl/fl
SA254677	A35096_tumor_Control	Tumor	Arg1fl/fl
SA254678	A35466_tumor_Arg1_KO	Tumor	Lyz2-Cre+/+; Arg1fl/fl
SA254679	A35469_tumor_Arg1_KO	Tumor	Lyz2-Cre+/+; Arg1fl/fl
SA254680	A35465_tumor_Arg1_KO	Tumor	Lyz2-Cre+/+; Arg1fl/fl
SA254681	0788_tumor_Arg1_KO	Tumor	Lyz2-Cre+/+; Arg1fl/fl
SA254682	0785_tumor_Arg1_KO	Tumor	Lyz2-Cre+/+; Arg1fl/fl
SA254683	0787_tumor_Arg1_KO	Tumor	Lyz2-Cre+/+; Arg1fl/fl
SA254684	0789_tumor_Arg1_KO	Tumor	Lyz2-Cre+/+; Arg1fl/fl
SA254685	A35089_tumor_Arg1_KO	Tumor	Lyz2-Cre+/+; Arg1fl/fl

Showing results 1 to 55 of 55

Showing results 1 to 55 of 55

Collection:

Collection ID:	CO002622
Collection Summary:	6~8-month-old female & male Lyz2-Cre +/+; Arg1fl/fl and litter mate control Arg1fl/fl mice with murine PDAC orthotopic tumors underwent dual jugular vein & carotid artery catheterization surgery. On day 5 of post recovery, mice received a 0.28 mg/g 10 min. bolus followed by a continuous 4 hr. infusion 0.005 mg/g/min infusion of 15N2-glutamine (Cambridge Isotope Laboratory #NLM-1328-PK). Plasma samples were taken at time points: 0' 15' 30' 60' 120' 180’ 240’. Tumors and tissues were harvested at 240’ and immediately snap frozen with liquid nitrogen stored at -80°C prior to analysis.
Sample Type:	Tumor, plasma

Treatment:

Treatment ID:	TR002641
Treatment Summary:	6~8-month-old female & male Lyz2-Cre +/+; Arg1fl/fl and litter mate control Arg1fl/fl mice with murine PDAC orthotopic tumors underwent dual jugular vein & carotid artery catheterization surgery. On day 5 of post recovery, mice received a 0.28 mg/g 10 min. bolus followed by a continuous 4 hr. infusion 0.005 mg/g/min infusion of 15N2-glutamine (Cambridge Isotope Laboratory #NLM-1328-PK). Plasma samples were taken at time points: 0' 15' 30' 60' 120' 180’ 240’. Tumors and tissues were harvested at 240’ and immediately snap frozen with liquid nitrogen stored at -80°C prior to analysis.

Treatment ID:

TR002641

Treatment Summary:

6~8-month-old female & male Lyz2-Cre +/+; Arg1fl/fl and litter mate control Arg1fl/fl mice with murine PDAC orthotopic tumors underwent dual jugular vein & carotid artery catheterization surgery. On day 5 of post recovery, mice received a 0.28 mg/g 10 min. bolus followed by a continuous 4 hr. infusion 0.005 mg/g/min infusion of 15N2-glutamine (Cambridge Isotope Laboratory #NLM-1328-PK). Plasma samples were taken at time points: 0' 15' 30' 60' 120' 180’ 240’. Tumors and tissues were harvested at 240’ and immediately snap frozen with liquid nitrogen stored at -80°C prior to analysis.

Sample Preparation:

Sampleprep ID:	SP002635
Sampleprep Summary:	Cryogenically frozen tumor pieces were ground to a fine homogenous powder with a liquid nitrogen cooled mortar and pestle. ~30mg of tissue powder was weighed into sample tubes, and metabolites were extracted with 600µL HPLC grade methanol, 300µL HPLC grade water, and 400µL chloroform. Samples were vortexed for 10min at 4°C, centrifuged 21,000xg at 4°C for 10 min. 400µL of the aqueous top layer was removed into a new tube and dried under nitrogen. Dried tumor extracts were resuspended in 100µL HPLC grade water and LC-MS analysis was performed as described before(Sullivan et al., 2019b, 2019a). For plasma samples, we extracted polar metabolites from 5µL of sample using 45µL of a 75:25:0.1 HPLC grade acetonitrile:methanol:formic acid extraction mix. Samples in extraction mix were vortexed for 10 min at 4°C and centrifugated at 15,000x rpm for 10 min at 4°C to pellet insoluble material. 20µL of the soluble polar metabolite supernatant was moved to sample vials for analysis by LC-MS.

Sampleprep ID:

SP002635

Sampleprep Summary:

Cryogenically frozen tumor pieces were ground to a fine homogenous powder with a liquid nitrogen cooled mortar and pestle. ~30mg of tissue powder was weighed into sample tubes, and metabolites were extracted with 600µL HPLC grade methanol, 300µL HPLC grade water, and 400µL chloroform. Samples were vortexed for 10min at 4°C, centrifuged 21,000xg at 4°C for 10 min. 400µL of the aqueous top layer was removed into a new tube and dried under nitrogen. Dried tumor extracts were resuspended in 100µL HPLC grade water and LC-MS analysis was performed as described before(Sullivan et al., 2019b, 2019a). For plasma samples, we extracted polar metabolites from 5µL of sample using 45µL of a 75:25:0.1 HPLC grade acetonitrile:methanol:formic acid extraction mix. Samples in extraction mix were vortexed for 10 min at 4°C and centrifugated at 15,000x rpm for 10 min at 4°C to pellet insoluble material. 20µL of the soluble polar metabolite supernatant was moved to sample vials for analysis by LC-MS.

Combined analysis:

Analysis ID	AN004163
Analysis type	MS
Chromatography type	HILIC
Chromatography system	Thermo Vanquish
Column	Waters Atlantis BEH Z-HILIC (150 x 2.1 mm, 2.5um)
MS Type	ESI
MS instrument type	Orbitrap
MS instrument name	Thermo Orbitrap IQ-X Tribrid
Ion Mode	UNSPECIFIED
Units	Natural abundance corrected percentages

Chromatography:

Chromatography ID:	CH003082
Instrument Name:	Thermo Vanquish
Column Name:	Waters Atlantis BEH Z-HILIC (150 x 2.1 mm, 2.5um)
Column Temperature:	30°C
Flow Gradient:	0 minute: 85% B, 0.5 minute: 85% B, 18 minutes: 20% B, 20 minutes: 20% B, 20.5 minutes: 85% B and 28 minutes: 85% B
Flow Rate:	0.2 mL/minute
Solvent A:	20 mM ammonium bicarbonate at pH 9.6, adjusted by ammonium hydroxide addition
Solvent B:	100% Acetonitrile
Chromatography Type:	HILIC

MS:

MS ID:	MS003910
Analysis ID:	AN004163
Instrument Name:	Thermo Orbitrap IQ-X Tribrid
Instrument Type:	Orbitrap
MS Type:	ESI
MS Comments:	Data acquisition was done using the Xcalibur software (Thermo Scientific) in full-scan mode with a range of 70-1000 m/z at 60K. Metabolite identification was done by matching the retention time and MS/MS fragmentation to the reference standards. Data analysis was performed using Tracefinder 5.1 software (Thermo Scientific).
Ion Mode:	UNSPECIFIED