Summary of Study ST000422

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 PR000330. The data can be accessed directly via it's Project DOI: 10.21228/M8W02Q 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	ST000422
Study Title	Type 1 Diabetes good glycemic control and controls samples
Study Type	Plasma metabolites in T1 diabetes
Study Summary	The objective of the study was to determine whether T1D with good glycemic control have persistent abnormalities of metabolites and pathways that exist in T1D with poor glycemic control.
Institute	Mayo Clinic
Department	Endocrinology
Laboratory	Mayo Clinic Metabolomics Resource Core
Last Name	Nair
First Name	Sreekumaran
Address	200 First Street SW, Rochester, MN 55905
Email	Nair.K@mayo.edu
Phone	507-285-2415
Submit Date	2016-07-01
Raw Data Available	Yes
Raw Data File Type(s)	d
Analysis Type Detail	LC-MS
Release Date	2016-09-23
Release Version	1

Select appropriate tab below to view additional metadata details:

Project:

Project ID:	PR000330
Project DOI:	doi: 10.21228/M8W02Q
Project Title:	Impact of Long-Term Poor and Good Glycemic Control on Metabolomics Alterations in Type 1 Diabetic People.
Project Type:	Untargeted LC-MS Metabolomics
Project Summary:	The objective of the study was to determine whether T1D with good glycemic control have persistent abnormalities of metabolites and pathways that exist in T1D with poor glycemic control.
Institute:	Mayo Clinic
Department:	Endocrinology
Laboratory:	Mayo Clinic Metabolomics Resource Core
Last Name:	Nair
First Name:	Sreekumaran
Address:	200 First Street SW, Rochester, MN 55905
Email:	Nair.K@mayo.edu
Phone:	507-285-2415

Subject:

Subject ID:	SU000443
Subject Type:	Animal
Subject Species:	Homo sapiens
Taxonomy ID:	9606
Species Group:	Human

Factors:

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

mb_sample_id	local_sample_id	treatment
SA021357	08feb12_56-r002.d	ND
SA021358	08feb12_80-r001.d	ND
SA021359	08feb12_56-r001.d	ND
SA021360	08feb12_45-r001.d	ND
SA021361	08feb12_43-r002.d	ND
SA021362	08feb12_80-r002.d	ND
SA021363	08feb12_45-r002.d	ND
SA021364	08feb12_59-r001.d	ND
SA021365	08feb12_62-r001.d	ND
SA021366	08feb12_62-r002.d	ND
SA021367	08feb12_81-r002.d	ND
SA021368	08feb12_81-r001.d	ND
SA021369	08feb12_59-r002.d	ND
SA021370	08feb12_43-r001.d	ND
SA021371	08feb12_39-r002.d	ND
SA021372	08feb12_22-r002.d	ND
SA021373	08feb12_24-r001.d	ND
SA021374	08feb12_22-r001.d	ND
SA021375	08feb12_15-r002.d	ND
SA021376	08feb12_13-r002.d	ND
SA021377	08feb12_15-r001.d	ND
SA021378	08feb12_24-r002.d	ND
SA021379	08feb12_26-r001.d	ND
SA021380	08feb12_39-r001.d	ND
SA021381	15feb12_13-r002.d	ND
SA021382	08feb12_28-r002.d	ND
SA021383	08feb12_28-r001.d	ND
SA021384	08feb12_26-r002.d	ND
SA021385	08feb12_41-r002.d	ND
SA021386	15feb12_22-r002.d	ND
SA021387	13feb12_39-r002.d	ND
SA021388	13feb12_41-r002.d	ND
SA021389	13feb12_28-r002.d	ND
SA021390	13feb12_26-r002.d	ND
SA021391	13feb12_22-r002.d	ND
SA021392	13feb12_24-r002.d	ND
SA021393	13feb12_43-r002.d	ND
SA021394	13feb12_45-r002.d	ND
SA021395	13feb12_81-r002.d	ND
SA021396	13feb12_62-r002.d	ND
SA021397	13feb12_59-r002.d	ND
SA021398	13feb12_80-r002.d	ND
SA021399	13feb12_56-r002.d	ND
SA021400	13feb12_15-r002.d	ND
SA021401	13feb12_13-r002.d	ND
SA021402	15feb12_39-r002.d	ND
SA021403	15feb12_41-r002.d	ND
SA021404	15feb12_28-r002.d	ND
SA021405	15feb12_26-r002.d	ND
SA021406	08feb12_13-r001.d	ND
SA021407	15feb12_24-r002.d	ND
SA021408	15feb12_43-r002.d	ND
SA021409	15feb12_45-r002.d	ND
SA021410	15feb12_81-r002.d	ND
SA021411	15feb12_62-r002.d	ND
SA021412	15feb12_59-r002.d	ND
SA021413	15feb12_80-r002.d	ND
SA021414	15feb12_56-r002.d	ND
SA021415	15feb12_15-r002.d	ND
SA021416	08feb12_41-r001.d	ND
SA021417	10jan12_80-r002.d	ND
SA021418	10jan12_22-r002.d	ND
SA021419	10jan12_43-r002.d	ND
SA021420	10jan12_43-r001.d	ND
SA021421	10jan12_22-r001.d	ND
SA021422	10jan12_28-r002.d	ND
SA021423	10jan12_26-r001.d	ND
SA021424	10jan12_28-r001.d	ND
SA021425	10jan12_80-r001.d	ND
SA021426	10jan12_39-r002.d	ND
SA021427	10jan12_26-r002.d	ND
SA021428	10jan12_45-r001.d	ND
SA021429	10jan12_45-r002.d	ND
SA021430	10jan12_56-r001.d	ND
SA021431	10jan12_56-r002.d	ND
SA021432	10jan12_24-r001.d	ND
SA021433	10jan12_24-r002.d	ND
SA021434	10jan12_59-r002.d	ND
SA021435	10jan12_59-r001.d	ND
SA021436	10jan12_41-r001.d	ND
SA021437	10jan12_13-r002.d	ND
SA021438	10jan12_81-r002.d	ND
SA021439	10jan12_13-r001.d	ND
SA021440	10jan12_39-r001.d	ND
SA021441	10jan12_81-r001.d	ND
SA021442	10jan12_15-r001.d	ND
SA021443	10jan12_15-r002.d	ND
SA021444	10jan12_62-r001.d	ND
SA021445	10jan12_41-r002.d	ND
SA021446	10jan12_62-r002.d	ND
SA021447	15feb12_58-r002.d	T1D good glycemic control
SA021448	15feb12_60-r002.d	T1D good glycemic control
SA021449	15feb12_27-r002.d	T1D good glycemic control
SA021450	15feb12_38-r002.d	T1D good glycemic control
SA021451	15feb12_40-r002.d	T1D good glycemic control
SA021452	10jan12_38-r001.d	T1D good glycemic control
SA021453	15feb12_55-r002.d	T1D good glycemic control
SA021454	15feb12_44-r002.d	T1D good glycemic control
SA021455	10jan12_27-r002.d	T1D good glycemic control
SA021456	15feb12_42-r002.d	T1D good glycemic control

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Collection:

Collection ID:	CO000437
Collection Summary:	At 5:00 AM after an overnight fast, baseline blood samples were collected from study participants. Plasma samples were stored at 80°C until analysis.
Sample Type:	Blood. Plasma was isolated for MS analysis.

Treatment:

Treatment ID:	TR000457
Treatment Summary:	Participants were admitted to the Clinical Research Unit at St Mary’s Hospital (Rochester, Minnesota) the evening before the study and spent overnight in the Clinical Research Unit. The participants were given a standard meal on the evening of the admission after which they fasted overnight. Participants with T1D were treated with insulin as per their usual individual programs. At 5:00 AM after an overnight fast, baseline blood samples were collected from study participants. Plasma samples were stored at 80°C until analysis.

Treatment ID:

TR000457

Treatment Summary:

Participants were admitted to the Clinical Research Unit at St Mary’s Hospital (Rochester, Minnesota) the evening before the study and spent overnight in the Clinical Research Unit. The participants were given a standard meal on the evening of the admission after which they fasted overnight. Participants with T1D were treated with insulin as per their usual individual programs. At 5:00 AM after an overnight fast, baseline blood samples were collected from study participants. Plasma samples were stored at 80°C until analysis.

Sample Preparation:

Sampleprep ID:	SP000450
Sampleprep Summary:	Plasma quality-control samples used in the study were prepared from pooled plasma spiked with a selection of metabolites to mimic elevated levels of metabolites during I− (insulin withdrawn) condition. Plasma was spiked with a standard mixture (3:1 ratio of plasma to spiking solution) containing 100 μg/mL niacin, hypoxanthine, leucine, isoleucine, phenylalanine, tryptophan, citric acid, glucose, hippuric acid, and taurocholic acid dissolved in 1:1 acetonitrile/water. All plasma samples (200 μL) were thawed on ice at 4°C followed by deproteinization with methanol (1:4 ratio of plasma to methanol) and vortexed for 10 s, followed by incubation at −20°C for 2 h. The samples were then centrifuged at 15,871g for 30 min at 4°C. The supernatants were lyophilized (Savant, Holbrook, NY) and stored at −20°C prior to analysis. The samples were reconstituted in 50% H2O/acetonitrile and passed through a Microcon YM3 filter (Millipore Corporation). The supernatants were transferred to analytical vials, stored in the autosampler at 4°C, and analyzed within 48 h of reconstitution in buffer.

Sampleprep ID:

SP000450

Sampleprep Summary:

Plasma quality-control samples used in the study were prepared from pooled plasma spiked with a selection of metabolites to mimic elevated levels of metabolites during I− (insulin withdrawn) condition. Plasma was spiked with a standard mixture (3:1 ratio of plasma to spiking solution) containing 100 μg/mL niacin, hypoxanthine, leucine, isoleucine, phenylalanine, tryptophan, citric acid, glucose, hippuric acid, and taurocholic acid dissolved in 1:1 acetonitrile/water. All plasma samples (200 μL) were thawed on ice at 4°C followed by deproteinization with methanol (1:4 ratio of plasma to methanol) and vortexed for 10 s, followed by incubation at −20°C for 2 h. The samples were then centrifuged at 15,871g for 30 min at 4°C. The supernatants were lyophilized (Savant, Holbrook, NY) and stored at −20°C prior to analysis. The samples were reconstituted in 50% H2O/acetonitrile and passed through a Microcon YM3 filter (Millipore Corporation). The supernatants were transferred to analytical vials, stored in the autosampler at 4°C, and analyzed within 48 h of reconstitution in buffer.

Combined analysis:

Analysis ID	AN000667	AN000668	AN000669	AN000670
Analysis type	MS	MS	MS	MS
Chromatography type	HILIC	HILIC	Reversed phase	Reversed phase
Chromatography system	Agilent 6220	Agilent 6220	Agilent 6220	Agilent 6220
Column	none	none	none	none
MS Type	ESI	ESI	ESI	ESI
MS instrument type	TOF	TOF	TOF	TOF
MS instrument name	Agilent 6220 TOF	Agilent 6220 TOF	Agilent 6220 TOF	Agilent 6220 TOF
Ion Mode	POSITIVE	NEGATIVE	POSITIVE	NEGATIVE
Units	intensity	intensity	intensity	intensity

Chromatography:

Chromatography ID:	CH000482
Chromatography Summary:	The liquid chromatography platform consisted of an Acquity UPLC system (Waters, Milford, MA). Plasma metabolite separation was achieved using both hydrophilic interaction chromatography (ethylene-bridged hybrid 2.1 × 150 mm, 1.7 μm; Waters) and reversed-phase liquid chromatography C18 (high-strength silica 2.1 × 150 mm, 1.8 μm; Waters). For each column, the run time was 20 min at a flow rate of 400 μL/min. Reverse-phase chromatography was performed using 99% solvent A (5 mmol/L NH4 acetate, 0.1% formic acid, and 1% acetonitrile) to 100% solvent B (95% acetonitrile with 0.1% formic acid). The gradient was 0 min, 0% B; 1 min, 0% B; 3 min, 5% B; 13.0 min, 100% B; 16 min, 100% B; 16.5 min, 0% B; and 20 min, 0% B. Other LC parameters were injection volume 5 μL and column temperature 50°C. Each sample was injected in triplicate with blank injections between each sample. Quality controls and standards were run at the beginning and end of the sequence.
Instrument Name:	Agilent 6220
Column Name:	none
Column Temperature:	50
Flow Gradient:	0 min, 0% B; 1 min, 0% B; 3 min, 5% B; 13.0 min, 100% B; 16 min, 100% B; 16.5 min, 0% B; and 20 min, 0% B.
Flow Rate:	400 µL/min
Solvent A:	1% acetonitrile/99% water; 0.1% formic acid; 5 mM ammonium acetate
Solvent B:	95% acetonitrile/5% water; 0.1% formic acid
Chromatography Type:	HILIC

Chromatography ID:	CH000483
Chromatography Summary:	The liquid chromatography platform consisted of an Acquity UPLC system (Waters, Milford, MA). Plasma metabolite separation was achieved using both hydrophilic interaction chromatography (ethylene-bridged hybrid 2.1 × 150 mm, 1.7 μm; Waters) and reversed-phase liquid chromatography C18 (high-strength silica 2.1 × 150 mm, 1.8 μm; Waters). For each column, the run time was 20 min at a flow rate of 400 μL/min. Reverse-phase chromatography was performed using 99% solvent A (5 mmol/L NH4 acetate, 0.1% formic acid, and 1% acetonitrile) to 100% solvent B (95% acetonitrile with 0.1% formic acid). The gradient was 0 min, 0% B; 1 min, 0% B; 3 min, 5% B; 13.0 min, 100% B; 16 min, 100% B; 16.5 min, 0% B; and 20 min, 0% B. Other LC parameters were injection volume 5 μL and column temperature 50°C. Each sample was injected in triplicate with blank injections between each sample. Quality controls and standards were run at the beginning and end of the sequence.
Instrument Name:	Agilent 6220
Column Name:	none
Column Temperature:	50
Flow Gradient:	0 min, 0% B; 1 min, 0% B; 3 min, 5% B; 13.0 min, 100% B; 16 min, 100% B; 16.5 min, 0% B; and 20 min, 0% B.
Flow Rate:	400 µL/min
Solvent A:	99% water/1% acetonitrile; 0.1% formic acid; 5 mM ammonium acetate
Solvent B:	95% acetonitrile/5% water; 0.1% formic acid
Chromatography Type:	Reversed phase

MS:

MS ID:	MS000593
Analysis ID:	AN000667
Instrument Name:	Agilent 6220 TOF
Instrument Type:	TOF
MS Type:	ESI
Ion Mode:	POSITIVE
Capillary Temperature:	300°C
Capillary Voltage:	3.5 kV
Fragment Voltage:	150 V
Mass Accuracy:	<5 parts per million and ~20000 respectively
Nebulizer:	nebulizer gas 325°C
Octpole Voltage:	250 V
Scan Range Moverz:	50-1200
Scanning Cycle:	0.5 s
Skimmer Voltage:	58 V

MS ID:	MS000594
Analysis ID:	AN000668
Instrument Name:	Agilent 6220 TOF
Instrument Type:	TOF
MS Type:	ESI
Ion Mode:	NEGATIVE
Capillary Temperature:	300°C
Capillary Voltage:	3.5 kV
Fragment Voltage:	150 V
Mass Accuracy:	<5 parts per million and ~20000 respectively
Nebulizer:	nebulizer gas 325°C
Octpole Voltage:	250 V
Scan Range Moverz:	50-1200
Scanning Cycle:	0.5 s
Skimmer Voltage:	58 V

MS ID:	MS000595
Analysis ID:	AN000669
Instrument Name:	Agilent 6220 TOF
Instrument Type:	TOF
MS Type:	ESI
Ion Mode:	POSITIVE
Capillary Temperature:	300°C
Capillary Voltage:	3.5 kV
Fragment Voltage:	150 V
Mass Accuracy:	<5 parts per million and ~20000 respectively
Nebulizer:	nebulizer gas 325°C
Octpole Voltage:	250 V
Scan Range Moverz:	50-1200
Scanning Cycle:	0.5 s
Skimmer Voltage:	58 V

MS ID:	MS000596
Analysis ID:	AN000670
Instrument Name:	Agilent 6220 TOF
Instrument Type:	TOF
MS Type:	ESI
Ion Mode:	NEGATIVE
Capillary Temperature:	300°C
Capillary Voltage:	3.5 kV
Fragment Voltage:	150 V
Mass Accuracy:	<5 parts per million and ~20000 respectively
Nebulizer:	nebulizer gas 325°C
Octpole Voltage:	250 V
Scan Range Moverz:	50-1200
Scanning Cycle:	0.5 s
Skimmer Voltage:	58 V