Summary of Study ST002125
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 PR001348. The data can be accessed directly via it's Project DOI: 10.21228/M8GD8D 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 | ST002125 |
| Study Title | Amino acids and TCA substrates in hematopoietic cells (Part2) |
| Study Summary | This study uses [13C,15N] labeled amino acids to study the amino acid consumption and their catabolism into tricarboxylic acid cycle substrates in hematopoietic stem cells, hemopoietic progenitors, and differentiated hematopoietic cells under different conditions, such as homeostasis and proliferation and with drug treatment. |
| Institute | Sun Yat-sen University |
| Last Name | Zhao |
| First Name | Meng |
| Address | Zhongshan 2nd Road |
| zhaom38@mail.sysu.edu.cn | |
| Phone | 18138799889 |
| Submit Date | 2022-04-06 |
| Raw Data Available | Yes |
| Raw Data File Type(s) | cdf |
| Analysis Type Detail | GC-MS |
| Release Date | 2022-11-01 |
| Release Version | 1 |
Select appropriate tab below to view additional metadata details:
Project:
| Project ID: | PR001348 |
| Project DOI: | doi: 10.21228/M8GD8D |
| Project Title: | Amino acid catabolism in hematopoietic cells |
| Project Summary: | Hematopoietic stem cells (HSCs) adapt their metabolism to maintenance and proliferation, but the mechanism remains incompletely understood. Here, we have investigated the total levels, uptake and catabolism of amino acid in hematopoietic stem cells, hemopoietic progenitors, and differentiated hematopoietic cells. We have also studied the catabolism of amino acid in hematopoietic stem cells under different conditions, such as homeostasis and proliferation and with drug treatment. Moreover, glycolytic metabolite, NAD+ precursor nicotinamide riboside (NR), accelerated AA catabolism to activate GCN2 and sustain long-term function of HSCs. Overall, our study uncovers the direct links between metabolic alterations and translation control in HSCs during homeostasis and proliferation. |
| Institute: | Sun Yat-sen University |
| Last Name: | Zhao |
| First Name: | Meng |
| Address: | Zhongshan 2nd Road |
| Email: | zhaom38@mail.sysu.edu.cn |
| Phone: | 18138799889 |
Subject:
| Subject ID: | SU002210 |
| 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 | Source_Name[gating] | Treatment | Batch | Note |
|---|---|---|---|---|---|
| SA204320 | BM_supernatant_5FU_1 | Bone marrow supernatant | 5 FU 2 weeks | 1c | Unlabeled AAs were used for total AA (FigS2.D) |
| SA204321 | BM_supernatant_5FU_2 | Bone marrow supernatant | 5 FU 2 weeks | 1c | Unlabeled AAs were used for total AA (FigS2.D) |
| SA204322 | BM_supernatant_5FU_3 | Bone marrow supernatant | 5 FU 2 weeks | 1c | Unlabeled AAs were used for total AA (FigS2.D) |
| SA204323 | BM_supernatant_Ctrl_1 | Bone marrow supernatant | HSC Basal | 1c | Unlabeled AAs were used for total AA (FigS2.D) |
| SA204324 | BM_supernatant_Ctrl_2 | Bone marrow supernatant | HSC Basal | 1c | Unlabeled AAs were used for total AA (FigS2.D) |
| SA204325 | BM_supernatant_Ctrl_3 | Bone marrow supernatant | HSC Basal | 1c | Unlabeled AAs were used for total AA (FigS2.D) |
| SA204326 | HSC_5FU_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 1 h | 1c | [13C, 15N] AAs were used for AA uptake (Fig2.B, Fig5M); unlabeled AAs and TCA substrate were used for total AA levels (Fig2.C, Fig5K) and TCA substrate levels (Fig2.K, Fig5J). |
| SA204327 | HSC_5FU_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 1 h | 1c | [13C, 15N] AAs were used for AA uptake (Fig2.B, Fig5M); unlabeled AAs and TCA substrate were used for total AA levels (Fig2.C, Fig5K) and TCA substrate levels (Fig2.K, Fig5J). |
| SA204328 | HSC_5FU_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 1 h | 1c | [13C, 15N] AAs were used for AA uptake (Fig2.B, Fig5M); unlabeled AAs and TCA substrate were used for total AA levels (Fig2.C, Fig5K) and TCA substrate levels (Fig2.K, Fig5J). |
| SA204329 | HSC_5FU_0h_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 0 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204330 | HSC_5FU_0h_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 0 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204331 | HSC_5FU_0h_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 0 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204332 | HSC_5FU_12h_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 12 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204333 | HSC_5FU_12h_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 12 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204334 | HSC_5FU_12h_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 12 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204335 | HSC_5FU_6h_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 6 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204336 | HSC_5FU_6h_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 6 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204337 | HSC_5FU_6h_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | 5 FU 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 6 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204338 | HSC_Cultured_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 1 h | 1c | [13C, 15N] AAs were used for AA uptake (Fig2.B); unlabeled AAs and TCA substrate were used for total AA levels (Fig2.C) and TCA substrate levels (Fig2.K). |
| SA204339 | HSC_Cultured_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 1 h | 1c | [13C, 15N] AAs were used for AA uptake (Fig2.B); unlabeled AAs and TCA substrate were used for total AA levels (Fig2.C) and TCA substrate levels (Fig2.K). |
| SA204340 | HSC_Cultured_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 1 h | 1c | [13C, 15N] AAs were used for AA uptake (Fig2.B); unlabeled AAs and TCA substrate were used for total AA levels (Fig2.C) and TCA substrate levels (Fig2.K). |
| SA204341 | HSC_Cultured_6h_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 0 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204342 | HSC_Cultured_0h_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 0 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204343 | HSC_Cultured_0h_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 0 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204344 | HSC_Cultured_0h_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 0 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204345 | HSC_Cultured_12h_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 12 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204346 | HSC_Cultured_12h_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 12 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204347 | HSC_Cultured_12h_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 12 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204348 | HSC_Cultured_6h_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 6 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204349 | HSC_Cultured_6h_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | Ex vivo culture 2 weeks, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 6 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig2.D). |
| SA204353 | HSC_Ctrl_0h_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 0 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig1.C, Fig2.D). |
| SA204354 | HSC_Ctrl_0h_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 0 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig1.C, Fig2.D). |
| SA204355 | HSC_Ctrl_0h_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 0 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig1.C, Fig2.D). |
| SA204356 | HSC_Ctrl_12h_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 12 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig1.C, Fig2.D). |
| SA204357 | HSC_Ctrl_12h_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 12 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig1.C, Fig2.D). |
| SA204358 | HSC_Ctrl_12h_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 12 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig1.C, Fig2.D). |
| SA204359 | HSC_Ctrl_6h_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 6 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig1.C, Fig2.D). |
| SA204360 | HSC_Ctrl_6h_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 6 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig1.C, Fig2.D). |
| SA204361 | HSC_Ctrl_6h_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal, [13C, 15N] AAs were incorporated for 24 h and subsequently washed out for 6 h | 1b | [13C, 15N] AA levels and [13C]TCA substrate levels in different time point were calculated for AA catabolism (Fig1.C, Fig2.D). |
| SA204350 | HSC_Ctrl_3 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal or Ctrl, [13C, 15N] AAs were incorporated for 1 h | 1c | [13C, 15N] AAs were used for AA uptake (Fig2.B, Fig5M); unlabeled AAs and TCA substrate were used for total AA levels (Fig2.C, Fig5K) and TCA substrate levels (Fig2.K, Fig5J). |
| SA204351 | HSC_Ctrl_1 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal or Ctrl, [13C, 15N] AAs were incorporated for 1 h | 1c | [13C, 15N] AAs were used for AA uptake (Fig2.B, Fig5M); unlabeled AAs and TCA substrate were used for total AA levels (Fig2.C, Fig5K) and TCA substrate levels (Fig2.K, Fig5J). |
| SA204352 | HSC_Ctrl_2 | Lin– Scal1+ c-Kit+ CD48– CD150+ (HSC) | HSC Basal or Ctrl, [13C, 15N] AAs were incorporated for 1 h | 1c | [13C, 15N] AAs were used for AA uptake (Fig2.B, Fig5M); unlabeled AAs and TCA substrate were used for total AA levels (Fig2.C, Fig5K) and TCA substrate levels (Fig2.K, Fig5J). |
| Showing results 1 to 42 of 42 |
Collection:
| Collection ID: | CO002203 |
| Collection Summary: | 5×10^5 indicated cells were incubated with 100 µM stable [13C,15N] amino acids (MSK-A2-US-1.2, Cambridge Isotope Laboratories) for indicated time and centrifuged at 500 g for 5 min at 4 °C. The pelleted cells were extracted in 500 µl ice-cold Acetonitrile: Isopropyl Alcohol: water (3:3:2 v/v/v) and aliquoted as three technical replicates. The extracts were vortexed for 5 min at 4 °C and centrifuged at 14,000 g for 2 min at 4 °C. The supernatants were dried by vacuum spin for subsequent derivatization and stored at -20 ℃. |
| Sample Type: | Bone marrow |
Treatment:
| Treatment ID: | TR002222 |
| Treatment Summary: | Germ-free C57BL/6J mice were intraperitoneally injected with 10 mg/kg 5FU (F6627-5G, Sigma-Aldrich) for 14 days, or fed with vehicle or NR (400 mg/kg per day) (1341-23-7, ziyi-reagent) for consecutive 8 weeks (long-term) or 1 week (short-term). Hematopoietic cells were stained and sorted from treated mice. |
Sample Preparation:
| Sampleprep ID: | SP002216 |
| Sampleprep Summary: | To get the corresponding derivatives, the dried aliquots were incubated with 20 µL 2% (w/v) methoxyamine hydrochloride (226904, Sigma-Aldrich) in pyridine for 60 min at 37 °C, and silylated by 30 µL of N-Methyl-N-(tert-butyldimethylsilyl) trifluoroacetamide with 1% tert-Butyldimethylchlorosilane (TBDMS, 18162-48-6, Regis Technologies) for 30 min at 45 °C. The corresponding derivatives were analyzed by GC-MS using the Trace 1310 gas chromatograph (Thermo Fisher) with the DB-35ms column (Agilent Technologies) connected to the Q ExactiveTM GC OrbitrapTM GC-MS/MS system (Thermo Fisher). |
Combined analysis:
| Analysis ID | AN003478 |
|---|---|
| Analysis type | MS |
| Chromatography type | GC |
| Chromatography system | TRACE 1310 |
| Column | DB-35ms |
| MS Type | EI |
| MS instrument type | Orbitrap |
| MS instrument name | Thermo Q Exactive Orbitrap |
| Ion Mode | POSITIVE |
| Units | Peak Area |
Chromatography:
| Chromatography ID: | CH002567 |
| Instrument Name: | TRACE 1310 |
| Column Name: | DB-35ms |
| Chromatography Type: | GC |
MS:
| MS ID: | MS003239 |
| Analysis ID: | AN003478 |
| Instrument Name: | Thermo Q Exactive Orbitrap |
| Instrument Type: | Orbitrap |
| MS Type: | EI |
| MS Comments: | GC-MS data was acquired on Q-Exactive Orbitrap mass spectrometer (Thermo Fisher) coupled with Gas Chromatograph system TRACE 1310 (Thermo Fisher). Chromatographic separation was performed on a DB-35ms column module (30 m length x 0.25 mm internal diameter, Agilent Technologies). The column temperature was programmed with an initial temperature of 50 °C for 2 min, then ramped at 10°C/min to 325 °C, and maintained for 5 min. The mass range was set as 50-600 m/z, and the resolution was 60,000. The ion source temperature was 300°C with the transfer line temperature of 250°C, and the electron energy was 70 eV with EI source. |
| Ion Mode: | POSITIVE |
