Summary of Study ST003109

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 PR001915. The data can be accessed directly via it's Project DOI: 10.21228/M86137 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.

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Study ID	ST003109
Study Title	HZV029 Metabolomics
Study Summary	In this study, plasma samples were processed using an in-house one phase extraction protocol as previously published (Siddiqa, A., et al., A pilot metabolomic study of drug interaction with the immune response to seasonal influenza vaccination. npj Vaccines, 2023. 8(1): p. 92. ). The resulting extract was then analyzed on a Thermo ScientificTM TranscendTM Duo LX-2 UHPLC system interfaced with high resolution Thermo ScientificTM Orbitrap ID-XTM TribidTM mass spectrometer with a HESI ionization source. This dataset was collected over 17 batches and was used to evaluate the QA/QC metrics produced by the pipeline and resulting MS2 annotations generated from a complimentary AcquireX (deep scan) MS2 dataset were compared to compound discoverer.
Institute	Jackson Laboratory for Genomic Medicine
Laboratory	Shuzhao Li Laboratory
Last Name	Joshua
First Name	Mitchell
Address	10 Discovery Dr, Farmington CT 06032
Email	joshua.mitchell@jax.org
Phone	8608372474
Submit Date	2024-02-15
Publications	Common data models to streamline metabolomics processing and annotation, and implementation in a Python pipeline Joshua Mitchell, Yuanye Chi, Maheshwor Thapa, Zhiqiang Pang, Jianguo Xia, Shuzhao Li doi: https://doi.org/10.1101/2024.02.13.580048
Raw Data Available	Yes
Raw Data File Type(s)	mzML
Analysis Type Detail	LC-MS
Release Date	2024-05-24
Release Version	1

Select appropriate tab below to view additional metadata details:

Project:

Project ID:	PR001915
Project DOI:	doi: 10.21228/M86137
Project Title:	Evaluation of a python-centric metabolomics data processing pipeline based on Asari.
Project Summary:	To standardize metabolomics data analysis and facilitate future computational developments, it is essential is have a set of well-defined templates for common data structures. Here we describe a collection of data structures involved in metabolomics data processing and illustrate how they are utilized in a full-featured Python-centric pipeline. We demonstrate the performance of the pipeline, and the details in annotation and quality control using large-scale LC-MS metabolomics and lipidomics data and LC-MS/MS data. Multiple previously published datasets are also reanalyzed to showcase its utility in biological data analysis. This pipeline allows users to streamline data processing, quality control, annotation, and standardization in an efficient and transparent manner. This work fills a major gap in the Python ecosystem for computational metabolomics. The uploaded datasets include previously unreleased datasets used for the evaluation of this pipeline including two large plasma datasets taken from recipients of one of two herpes zoster vaccines, analyzed as 17 separate batches, and a lipidomics dataset collected on a subset of these patients.
Institute:	Jackson Laboratory for Genomic Medicine
Laboratory:	Shuzhao Li Laboratory
Last Name:	Joshua
First Name:	Mitchell
Address:	10 Discovery Dr, Farmington CT 06032
Email:	joshua.mitchell@jax.org
Phone:	8608372474
Funding Source:	NIH grants U01 CA235493 (NCI), R01 AI149746 and AI149746 S1 (NIAID), and UM1 HG012651 (NHGRI).
Publications:	Common data models to streamline metabolomics processing and annotation, and implementation in a Python pipeline (BioRxiv) Joshua Mitchell, Yuanye Chi, Maheshwor Thapa, Zhiqiang Pang, Jianguo Xia, Shuzhao Li; doi: https://doi.org/10.1101/2024.02.13.580048
Contributors:	Joshua Mitchell, Yuanye Chi, Maheshwor Thapa, Shuzhao Li

Subject:

Subject ID:	SU003224
Subject Type:	Human
Subject Species:	Homo sapiens
Taxonomy ID:	9606

Factors:

Subject type: Human; Subject species: Homo sapiens (Factor headings shown in green)

mb_sample_id	local_sample_id	Factor	Sample source
SA333736	raw_batch12_08062021_MT___Blank_20210806_003	blank	Process Blank
SA333737	raw_batch12_08062021_MT___Blank_20210806_004	blank	Process Blank
SA333738	raw_batch12_08062021_MT___Blank_20210806_002	blank	Process Blank
SA333739	raw_batch12_08062021_MT___Blank_20210806_001	blank	Process Blank
SA333740	raw_batch11_08052021_MT___Blank_20210805_006	blank	Process Blank
SA333741	raw_batch12_08062021_MT___Blank_20210806_005	blank	Process Blank
SA333742	raw_batch13_08072021_MT___Blank_20210807_001	blank	Process Blank
SA333743	raw_batch13_08072021_MT___Blank_20210807_004	blank	Process Blank
SA333744	raw_batch13_08072021_MT___Blank_20210807_005	blank	Process Blank
SA333745	raw_batch13_08072021_MT___Blank_20210807_003	blank	Process Blank
SA333746	raw_batch13_08072021_MT___Blank_20210807_002	blank	Process Blank
SA333747	raw_batch11_08052021_MT___Blank_20210805_005	blank	Process Blank
SA333748	raw_batch12_08062021_MT___Blank_20210806_006	blank	Process Blank
SA333749	raw_batch11_08052021_MT___Blank_20210805_004	blank	Process Blank
SA333750	raw_batch10_08042021_MT___Blank_20210804_001	blank	Process Blank
SA333751	raw_batch10_08042021_MT___Blank_20210804_002	blank	Process Blank
SA333752	raw_batch9_08032021_MT___Blank_20210803_006	blank	Process Blank
SA333753	raw_batch9_08032021_MT___Blank_20210803_005	blank	Process Blank
SA333754	raw_batch9_08032021_MT___Blank_20210803_004	blank	Process Blank
SA333755	raw_batch10_08042021_MT___Blank_20210804_003	blank	Process Blank
SA333756	raw_batch10_08042021_MT___Blank_20210804_005	blank	Process Blank
SA333757	raw_batch11_08052021_MT___Blank_20210805_003	blank	Process Blank
SA333758	raw_batch11_08052021_MT___Blank_20210805_002	blank	Process Blank
SA333759	raw_batch11_08052021_MT___Blank_20210805_001	blank	Process Blank
SA333760	raw_batch10_08042021_MT___Blank_20210804_006	blank	Process Blank
SA333761	raw_batch13_08072021_MT___Blank_20210807_006	blank	Process Blank
SA333762	raw_batch14_08082021_MT___Blank_20210808_001	blank	Process Blank
SA333763	raw_batch16_08102021_MT___Blank_20210810_006	blank	Process Blank
SA333764	raw_batch17_08112021_MT___Blank_20210811_001	blank	Process Blank
SA333765	raw_batch16_08102021_MT___Blank_20210810_005	blank	Process Blank
SA333766	raw_batch16_08102021_MT___Blank_20210810_004	blank	Process Blank
SA333767	raw_batch16_08102021_MT___Blank_20210810_003	blank	Process Blank
SA333768	raw_batch17_08112021_MT___Blank_20210811_002	blank	Process Blank
SA333769	raw_batch17_08112021_MT___Blank_20210811_003	blank	Process Blank
SA333770	raw_batch1_07262021_MT___Blank_20210726_001	blank	Process Blank
SA333771	raw_batch17_08112021_MT___Blank_20210811_006	blank	Process Blank
SA333772	raw_batch17_08112021_MT___Blank_20210811_005	blank	Process Blank
SA333773	raw_batch17_08112021_MT___Blank_20210811_004	blank	Process Blank
SA333774	raw_batch16_08102021_MT___Blank_20210810_002_20210809134659	blank	Process Blank
SA333775	raw_batch16_08102021_MT___Blank_20210810_001_20210809134133	blank	Process Blank
SA333776	raw_batch14_08082021_MT___Blank_20210808_005	blank	Process Blank
SA333777	raw_batch14_08082021_MT___Blank_20210808_006	blank	Process Blank
SA333778	raw_batch14_08082021_MT___Blank_20210808_004	blank	Process Blank
SA333779	raw_batch14_08082021_MT___Blank_20210808_003	blank	Process Blank
SA333780	raw_batch14_08082021_MT___Blank_20210808_002	blank	Process Blank
SA333781	raw_batch15_08092021_MT___Blank_20210809_001	blank	Process Blank
SA333782	raw_batch15_08092021_MT___Blank_20210809_002	blank	Process Blank
SA333783	raw_batch15_08092021_MT___Blank_20210809_006	blank	Process Blank
SA333784	raw_batch15_08092021_MT___Blank_20210809_005	blank	Process Blank
SA333785	raw_batch15_08092021_MT___Blank_20210809_004	blank	Process Blank
SA333786	raw_batch15_08092021_MT___Blank_20210809_003	blank	Process Blank
SA333787	raw_batch9_08032021_MT___Blank_20210803_003	blank	Process Blank
SA333788	raw_batch10_08042021_MT___Blank_20210804_004	blank	Process Blank
SA333789	raw_batch3_07292021_MT___Blank_20210728_003	blank	Process Blank
SA333790	raw_batch3_07292021_MT___Blank_20210728_004	blank	Process Blank
SA333791	raw_batch3_07292021_MT___Blank_20210728_002	blank	Process Blank
SA333792	raw_batch3_07292021_MT___Blank_20210728_001	blank	Process Blank
SA333793	raw_batch2_07272021_MT___Blank_20210727_006	blank	Process Blank
SA333794	raw_batch9_08032021_MT___Blank_20210803_002	blank	Process Blank
SA333795	raw_batch3_07292021_MT___Blank_20210728_006	blank	Process Blank
SA333796	raw_batch4_07302021_MT___Blank_20210729_004	blank	Process Blank
SA333797	raw_batch4_07302021_MT___Blank_20210729_005	blank	Process Blank
SA333798	raw_batch4_07302021_MT___Blank_20210729_003	blank	Process Blank
SA333799	raw_batch4_07302021_MT___Blank_20210729_002_20210729173910	blank	Process Blank
SA333800	raw_batch4_07302021_MT___Blank_20210729_001_20210729173052	blank	Process Blank
SA333801	raw_batch2_07272021_MT___Blank_20210727_005	blank	Process Blank
SA333802	raw_batch2_07272021_MT___Blank_20210727_004	blank	Process Blank
SA333803	raw_batch1_07262021_MT___Blank_20210726_003	blank	Process Blank
SA333804	raw_batch1_07262021_MT___Blank_20210726_004	blank	Process Blank
SA333805	raw_batch1_07262021_MT___Blank_20210726_002B	blank	Process Blank
SA333806	raw_batch1_07262021_MT___Blank_20210726_001A	blank	Process Blank
SA333807	raw_batch1_07262021_MT___Blank_20210726_002	blank	Process Blank
SA333808	raw_batch1_07262021_MT___Blank_20210726_005	blank	Process Blank
SA333809	raw_batch1_07262021_MT___Blank_20210726_006	blank	Process Blank
SA333810	raw_batch2_07272021_MT___Blank_20210727_002	blank	Process Blank
SA333811	raw_batch2_07272021_MT___Blank_20210727_003	blank	Process Blank
SA333812	raw_batch2_07272021_MT___Blank_20210727_001	blank	Process Blank
SA333813	raw_batch1_07262021_MT___Blank_20210726_008	blank	Process Blank
SA333814	raw_batch1_07262021_MT___Blank_20210726_007	blank	Process Blank
SA333815	raw_batch4_07302021_MT___Blank_20210729_006	blank	Process Blank
SA333816	raw_batch3_07292021_MT___Blank_20210728_005	blank	Process Blank
SA333817	raw_batch7_08012021_MT___Blank_20210801_006	blank	Process Blank
SA333818	raw_batch8_08022021_MT___Blank_20210802_001_20210802210939	blank	Process Blank
SA333819	raw_batch7_08012021_MT___Blank_20210801_005	blank	Process Blank
SA333820	raw_batch7_08012021_MT___Blank_20210801_004	blank	Process Blank
SA333821	raw_batch7_08012021_MT___Blank_20210801_003	blank	Process Blank
SA333822	raw_batch5_07302021_MT___Blank_20210730_001	blank	Process Blank
SA333823	raw_batch8_08022021_MT___Blank_20210802_003	blank	Process Blank
SA333824	raw_batch9_08032021_MT___Blank_20210803_001	blank	Process Blank
SA333825	raw_batch8_08022021_MT___Blank_20210802_006	blank	Process Blank
SA333826	raw_batch8_08022021_MT___Blank_20210802_005	blank	Process Blank
SA333827	raw_batch8_08022021_MT___Blank_20210802_004	blank	Process Blank
SA333828	raw_batch7_08012021_MT___Blank_20210801_002	blank	Process Blank
SA333829	raw_batch8_08022021_MT___Blank_20210802_002	blank	Process Blank
SA333830	raw_batch5_07302021_MT___Blank_20210730_004	blank	Process Blank
SA333831	raw_batch5_07302021_MT___Blank_20210730_006	blank	Process Blank
SA333832	raw_batch5_07302021_MT___Blank_20210730_003	blank	Process Blank
SA333833	raw_batch5_07302021_MT___Blank_20210730_002	blank	Process Blank
SA333834	raw_batch7_08012021_MT___Blank_20210801_001	blank	Process Blank
SA333835	raw_batch6_07312021_MT___Blank_20210731_001	blank	Process Blank

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Collection:

Collection ID:	CO003217
Collection Summary:	Deidentified human plasma samples were used for this study: a) commercial Qstd and NIST plasma pool ; b) biosamples (from 1R01AI149746 (NIH-NIAID) samples) plasma, collected through venipuncture.
Sample Type:	Blood (plasma)
Storage Conditions:	-80℃

Treatment:

Treatment ID:	TR003233
Treatment Summary:	Not applicable.

Sample Preparation:

Sampleprep ID:	SP003230
Sampleprep Summary:	The plasma samples were thawed in ice. Metabolites extraction were carried out by protein precipitation using extraction solvent, acetonitrile:methanol (8:1, v/v) containing 0.1% formic acid and isotope labelled Trimethyl-13C3]-caffeine, [13C5]-L-glutamic acid, [15N2]-Uracil, [15N,13C5]-L-methionine, [13C6]-D-glucose and [15N]-L-tyrosin as spike-in controls. 30 μl of plasma was taken and 60 μl of extraction solvent was added. All samples were vortexed and incubated with shaking at 1000 rpm for 10 min at 4°C followed by centrifugation at 4°C for 15 min at 15,000 rpm. The supernatant was transferred into mass spec vials and 2 μl injected into UHPLC-MS.

Sampleprep ID:

SP003230

Sampleprep Summary:

The plasma samples were thawed in ice. Metabolites extraction were carried out by protein precipitation using extraction solvent, acetonitrile:methanol (8:1, v/v) containing 0.1% formic acid and isotope labelled Trimethyl-13C3]-caffeine, [13C5]-L-glutamic acid, [15N2]-Uracil, [15N,13C5]-L-methionine, [13C6]-D-glucose and [15N]-L-tyrosin as spike-in controls. 30 μl of plasma was taken and 60 μl of extraction solvent was added. All samples were vortexed and incubated with shaking at 1000 rpm for 10 min at 4°C followed by centrifugation at 4°C for 15 min at 15,000 rpm. The supernatant was transferred into mass spec vials and 2 μl injected into UHPLC-MS.

Combined analysis:

Analysis ID	AN005091	AN005092
Analysis type	MS	MS
Chromatography type	HILIC	Reversed phase
Chromatography system	Thermo Vanquish	Thermo Vanquish
Column	Thermo Accucore HILIC (100 x 2.1mm,2.6um)	Hypersil GOLDTM RP column (3 μm, 2.1 mm × 50 mm)
MS Type	ESI	ESI
MS instrument type	Orbitrap	Orbitrap
MS instrument name	Thermo Orbitrap ID-X tribrid	Thermo Orbitrap ID-X tribrid
Ion Mode	POSITIVE	NEGATIVE
Units	peak intensity	peak intensity

Chromatography:

Chromatography ID:	CH003847
Chromatography Summary:	The chromatographic separations were performed using Thermo ScientificTM TranscendTM Duo LX-2 UHPLC system interfaced with high resolution Thermo ScientificTM Orbitrap ID-XTM TribidTM mass spectrometer with a HESI ionization source, using positive and negative ionization modes. All samples were maintained at 4 °C in the autosampler. Data were acquired using hydrophilic interaction liquid chromatography (HILIC) and reversed phase (RP) column in parallel both in positive and negative polarities in full scan mode with mass resolution of 120,000. An AccucoreTM−150-Amide HILIC column (2.6 μm, 2.1 mm × 50 mm) embedded with Accucore-150-Amide-HILIC guard column (10 × 2.1 mm, 2.6 μm) (Thermo Fisher Scientific, MA, USA. Cat. 16726-012105) and a Hypersil GOLDTM RP column (3 μm, 2.1 mm × 50 mm) embedded with Hypersil GOLDTM RP guard column (2.1 mm x 10 mm, 3 μm) (Thermo Fisher Scientific, MA, USA. Cat. 25003-012101) maintained at 45 °C were used for chromatographic separation. 10 mM ammonium acetate in acetonitrile:water (95:5, v/v) with 0.1% acetic acid as mobile phase A and 10 mM ammonium acetate in acetonitrile:water (50:50, v/v) with 0.1% acetic acid as mobile phase B were used for HILIC method. 0.1% formic acid in water and 0.1% formic acid in acetonitrile were used as mobile phase A and B respectively for RP acquisition. For HILIC acquisition, following gradient was applied at a flow rate of 0.55 ml/min: 0–0.1 min: 0% B, 0.10–5.0 min: 98% B, and 5 min for cleaning and equilibration of column. For RP column, following gradient was applied at a flow rate of 0.4 ml/min: 0–0.1 min: 0% B, 0.10–1.9 min: 60% B, 1.9–5.0 min: 98% B, and 5 min cleaning and column equilibration. This way the mass spec data for each sample was collected consecutively, carrying only one (either HILIC or RP) eluent to the MS for 5 min, while the other eluent was directed to the waste during washing and re-equilibration.
Instrument Name:	Thermo Vanquish
Column Name:	Thermo Accucore HILIC (100 x 2.1mm,2.6um)
Column Temperature:	45
Flow Gradient:	0–0.1 min: 0% B, 0.10–5.0 min: 98% B, and 5 min for cleaning and equilibration of column
Flow Rate:	0.55 ml/min
Solvent A:	95% acetonitrile/5% water; 10 mM ammonium acetate; 0.1% acetic acid
Solvent B:	50% acetonitrile/50% water; 10 mM ammonium acetate; 0.1% acetic acid
Chromatography Type:	HILIC

Chromatography ID:	CH003848
Chromatography Summary:	The chromatographic separations were performed using Thermo ScientificTM TranscendTM Duo LX-2 UHPLC system interfaced with high resolution Thermo ScientificTM Orbitrap ID-XTM TribidTM mass spectrometer with a HESI ionization source, using positive and negative ionization modes. All samples were maintained at 4 °C in the autosampler. Data were acquired using hydrophilic interaction liquid chromatography (HILIC) and reversed phase (RP) column in parallel both in positive and negative polarities in full scan mode with mass resolution of 120,000. An AccucoreTM−150-Amide HILIC column (2.6 μm, 2.1 mm × 50 mm) embedded with Accucore-150-Amide-HILIC guard column (10 × 2.1 mm, 2.6 μm) (Thermo Fisher Scientific, MA, USA. Cat. 16726-012105) and a Hypersil GOLDTM RP column (3 μm, 2.1 mm × 50 mm) embedded with Hypersil GOLDTM RP guard column (2.1 mm x 10 mm, 3 μm) (Thermo Fisher Scientific, MA, USA. Cat. 25003-012101) maintained at 45 °C were used for chromatographic separation. 10 mM ammonium acetate in acetonitrile:water (95:5, v/v) with 0.1% acetic acid as mobile phase A and 10 mM ammonium acetate in acetonitrile:water (50:50, v/v) with 0.1% acetic acid as mobile phase B were used for HILIC method. 0.1% formic acid in water and 0.1% formic acid in acetonitrile were used as mobile phase A and B respectively for RP acquisition. For HILIC acquisition, following gradient was applied at a flow rate of 0.55 ml/min: 0–0.1 min: 0% B, 0.10–5.0 min: 98% B, and 5 min for cleaning and equilibration of column. For RP column, following gradient was applied at a flow rate of 0.4 ml/min: 0–0.1 min: 0% B, 0.10–1.9 min: 60% B, 1.9–5.0 min: 98% B, and 5 min cleaning and column equilibration. This way the mass spec data for each sample was collected consecutively, carrying only one (either HILIC or RP) eluent to the MS for 5 min, while the other eluent was directed to the waste during washing and re-equilibration.
Instrument Name:	Thermo Vanquish
Column Name:	Hypersil GOLDTM RP column (3 μm, 2.1 mm × 50 mm)
Column Temperature:	45
Flow Gradient:	0–0.1 min: 0% B, 0.10–1.9 min: 60% B, 1.9–5.0 min: 98% B, and 5 min cleaning and column equilibration
Flow Rate:	0.4 ml/min
Solvent A:	100% water; 0.1% formic acid
Solvent B:	100% acetonitrile; 0.1% formic acid
Chromatography Type:	Reversed phase

MS:

MS ID:	MS004828
Analysis ID:	AN005091
Instrument Name:	Thermo Orbitrap ID-X tribrid
Instrument Type:	Orbitrap
MS Type:	ESI
MS Comments:	Mass spectrometry data were collected with the following MS settings: mass range, 80–1000 m/z; spray voltage, 3500 V (ESI + ), 2800 V (ESI−); sheath gas, 45 Arb; auxiliary gas, 20 Arb; sweep gas, 1 Arb; ion transfer tube temperature, 325 °C; vaporizer temperature, 325 °C; full scan mass resolution, 120,000 (MS1); normalized AGC target (%), 25; maximum injection time, 100 ms. Data dependent fragmentation (dd-MS/MS) parameters for each polarity as follows: isolation window (m/z), 1.2; stepped HCD collision energy (%), 20,40,80; dd-MS/MS resolution, 30,000; normalized AGC target (%), 20; maximum injection time (ms), 54; microscan, 1; cycle time (sec), 1.2. A full scan data-dependent MS2 (ddMS2) method was utilized to collect MS2 spectra for identification of compounds.
Ion Mode:	POSITIVE

MS ID:	MS004829
Analysis ID:	AN005092
Instrument Name:	Thermo Orbitrap ID-X tribrid
Instrument Type:	Orbitrap
MS Type:	ESI
MS Comments:	Mass spectrometry data were collected with the following MS settings: mass range, 80–1000 m/z; spray voltage, 3500 V (ESI + ), 2800 V (ESI−); sheath gas, 45 Arb; auxiliary gas, 20 Arb; sweep gas, 1 Arb; ion transfer tube temperature, 325 °C; vaporizer temperature, 325 °C; full scan mass resolution, 120,000 (MS1); normalized AGC target (%), 25; maximum injection time, 100 ms. Data dependent fragmentation (dd-MS/MS) parameters for each polarity as follows: isolation window (m/z), 1.2; stepped HCD collision energy (%), 20,40,80; dd-MS/MS resolution, 30,000; normalized AGC target (%), 20; maximum injection time (ms), 54; microscan, 1; cycle time (sec), 1.2. A full scan data-dependent MS2 (ddMS2) method was utilized to collect MS2 spectra for identification of compounds.
Ion Mode:	NEGATIVE