Summary of Study ST001913

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 PR000319. The data can be accessed directly via it's Project DOI: 10.21228/M8H029 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	ST001913
Study Title	Stool metabolomics in the New Hampshire Birth Cohort Study
Study Type	Untargeted and semi-targeted metabolomics analysis
Study Summary	This is a study of data collected from fecal samples from larger New Hampshire Birth Cohort Study (NHBCS). 1H NMR metabolomic profiling of 524 infant stool samples collected at 6 week - 3 year age was performed and spectra were binned (untargeted metabolomics). A set of host-microbiome co-metabolites were library matched in individual sample spectra and their relative concentrations were determined. This study investigated associations of the functional metabolic response of the microbial milieu of the infant gut with environmental and other factors.
Institute	University of North Carolina at Chapel Hill
Department	Nutrition
Laboratory	Metabolomics and Exposome Laboratory, Nutrition Research Institute, UNC Chapel Hill
Last Name	Sumner
First Name	Susan
Address	500 Laureate Way, Kannapolis, NC 28081
Email	susan_sumner@unc.edu
Phone	(919) 622-4456
Submit Date	2021-08-09
Num Groups	2
Total Subjects	524
Study Comments	The number of groups includes the QC samples, Total samples = 572
Raw Data Available	Yes
Analysis Type Detail	NMR
Release Date	2023-01-31
Release Version	1

Select appropriate tab below to view additional metadata details:

Project:

Project ID:	PR000319
Project DOI:	doi: 10.21228/M8H029
Project Title:	Metabolomics Changes in the feces of infants exposed to arsenic
Project Summary:	Exposure to arsenic (As) during the vulnerable window of fetal development and early childhood has shown significant clinical effects. In highly exposed populations, altered immunity is one of the most affected pathways and can lead to an elevated risk of infection and a pre-disposition to allergy/atopy. Since well water in the New Hampshire region has been determined to be a potential source of As exposure, this study includes mother-infant dyads living in the area, who obtain household water from private wells. This study seeks to determine if in utero and early life As exposure is related to increase occurrence of childhood: infections, allergy and atopy, and diminished vaccine response. It has been observed that the microbiome is an important mediator of immune impairment due to As exposure. Therefore, we will further investigate the relation between in utero and early life As exposure on the development of the infant intestinal microbiome in the first year of life. For this study fecal samples, from infants at risk of As exposure, were collected at 6 weeks and 12 months of age. Metabolomics data will allow for a more complete picture of the relationships between the microbiome, As exposure and immune function.
Institute:	Dartmouth College
Department:	Department of Epidemiology
Last Name:	Margaret
First Name:	Karagas
Address:	One Medical Center Road, 7927 HB, Rubin Building, Lebanon, NH 03756
Email:	Margaret.Karagas@Dartmouth.edu
Phone:	603-653-9010

Subject:

Subject ID:	SU001991
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	Sample type
SA177030	BD3_P1	Batch-QC
SA177031	BD2_P4	Batch-QC
SA177032	BD3_P2	Batch-QC
SA177033	BD3_P3	Batch-QC
SA177034	BD3_P4	Batch-QC
SA177035	BD2_P2	Batch-QC
SA177036	BD2_P1	Batch-QC
SA177037	BD1_P1	Batch-QC
SA177038	BD1_P2	Batch-QC
SA177039	BD1_P3	Batch-QC
SA177040	BD1_P4	Batch-QC
SA177041	BD4_P1	Batch-QC
SA177042	BD2_P3	Batch-QC
SA177043	BD6_P2	Batch-QC
SA177044	BD5_P4	Batch-QC
SA177045	BD6_P3	Batch-QC
SA177046	BD6_P4	Batch-QC
SA177047	BD4_P2	Batch-QC
SA177048	BD5_P3	Batch-QC
SA177049	BD6_P1	Batch-QC
SA177050	BD4_P4	Batch-QC
SA177051	BD5_P1	Batch-QC
SA177052	BD4_P3	Batch-QC
SA177053	BD5_P2	Batch-QC
SA177054	S_440	Sample
SA177055	S_441	Sample
SA177056	S_44	Sample
SA177057	S_438	Sample
SA177058	S_442	Sample
SA177059	S_437	Sample
SA177060	S_439	Sample
SA177061	S_449	Sample
SA177062	S_448	Sample
SA177063	S_436	Sample
SA177064	S_447	Sample
SA177065	S_446	Sample
SA177066	S_444	Sample
SA177067	S_445	Sample
SA177068	S_443	Sample
SA177069	S_420	Sample
SA177070	S_423	Sample
SA177071	S_425	Sample
SA177072	S_422	Sample
SA177073	S_421	Sample
SA177074	S_42	Sample
SA177075	S_45	Sample
SA177076	S_426	Sample
SA177077	S_427	Sample
SA177078	S_433	Sample
SA177079	S_434	Sample
SA177080	S_431	Sample
SA177081	S_430	Sample
SA177082	S_428	Sample
SA177083	S_429	Sample
SA177084	S_435	Sample
SA177085	S_461	Sample
SA177086	S_47	Sample
SA177087	S_470	Sample
SA177088	S_469	Sample
SA177089	S_468	Sample
SA177090	S_466	Sample
SA177091	S_467	Sample
SA177092	S_471	Sample
SA177093	S_472	Sample
SA177094	S_477	Sample
SA177095	S_478	Sample
SA177096	S_476	Sample
SA177097	S_475	Sample
SA177098	S_473	Sample
SA177099	S_474	Sample
SA177100	S_465	Sample
SA177101	S_464	Sample
SA177102	S_455	Sample
SA177103	S_456	Sample
SA177104	S_454	Sample
SA177105	S_453	Sample
SA177106	S_451	Sample
SA177107	S_452	Sample
SA177108	S_457	Sample
SA177109	S_458	Sample
SA177110	S_419	Sample
SA177111	S_463	Sample
SA177112	S_460	Sample
SA177113	S_46	Sample
SA177114	S_459	Sample
SA177115	S_450	Sample
SA177116	S_407	Sample
SA177117	S_38	Sample
SA177118	S_380	Sample
SA177119	S_379	Sample
SA177120	S_378	Sample
SA177121	S_376	Sample
SA177122	S_377	Sample
SA177123	S_381	Sample
SA177124	S_382	Sample
SA177125	S_387	Sample
SA177126	S_388	Sample
SA177127	S_386	Sample
SA177128	S_385	Sample
SA177129	S_383	Sample

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Collection:

Collection ID:	CO001984
Collection Summary:	Infant stool samples were collected at home using provided diapers, sealed in a separate polyethylene bag and frozen in a home freezer or kept chilled until transport. Samples were transported in a cooler with ice packs and brought to the routine 6-week post-partum visit within 24 hours of collection. Stool samples remained frozen until processing where they were thawed at 4 °C. Using sterile applicators, 0.5–1 g of stool was aliquoted into trace element-free cryovial tubes and then frozen at −80 °C in a biorepository
Sample Type:	Feces
Storage Conditions:	-80℃

Treatment:

Treatment ID:	TR002003
Treatment Summary:	NA

Sample Preparation:

Sampleprep ID:	SP001997
Sampleprep Summary:	De-identified stool aliquots were shipped on dry ice and immediately stored at -80 °C for metabolomics analysis. Samples were randomized into batches. For each batch, samples were thawed and ~150mg of stool was transferred to MagNA Lyser tubes after recording the weight, Samples were then homogenized with 50% acetonitrile in water by using the Omni Bead Disruptor (Omni International, GA, USA). Homogenized samples were centrifuged at 16000 rcf and the supernatant was separated into another tube. An aliquot (1000 uL, 100 mg equivalent of fecal mass) was transferred into Eppendorf tube and lyophilized overnight. The dried extract was reconstituted in 700 uL of NMR master mix (containing 0.2M phosphate, 0.5 mM DSS-d6, and 0.2% sodium azide), vortexed on a multitube vortexer at speed 5 for 2 min and centrifuged at 16000 rcf for 5 min. A 600 µl aliquot of the supernatant was transferred into a pre-labeled 5mm NMR tube for data acquisition on a 700 MHz spectrometer. Additionally, study pooled samples (created from randomly selected study samples) and batch pooled quality control (QC) samples were generated from supernatants of study samples and aliquots of supernatants were dried and reconstituted similar to study samples described above, and used for QC purposes.
Sampleprep Protocol Filename:	1. Dartmouth-Fecal Metabolomics_NMR_Batch2 Procedures
Processing Storage Conditions:	4℃
Extraction Method:	50% Acetonitrile in Water
Extract Storage:	-80℃
Sample Resuspension:	In phosphate buffer containing D2O

Analysis:

Analysis ID:	AN003111
Laboratory Name:	Metabolomics and Exposome Lab at UNC Nutrition Research Institute
Analysis Type:	NMR
Software Version:	TopSpin 3.5
Operator Name:	Wimal Pathmasiri
Detector Type:	NMR
Data Format:	fid, 1r
Results File:	4a._Dartmouth-Fecal_Metabolomics_NMR_Normalized_Binned_Data.txt
Units:	ppm

NMR:

NMR ID:	NM000214
Analysis ID:	AN003111
Instrument Name:	Avance III 700 MHz NMR Spectrometer
Instrument Type:	FT-NMR
NMR Experiment Type:	1D-1H
Field Frequency Lock:	3015 Hz, D2O
Standard Concentration:	0.5 mM
Spectrometer Frequency:	700 MHz
NMR Probe:	CP QCI/HPCN
NMR Solvent:	90% H2O, 10% D2O
NMR Tube Size:	5 mm
Shimming Method:	topshim
Pulse Sequence:	noesygppr1d
Water Suppression:	pre-saturation
Pulse Width:	14.59 us
Power Level:	12.3 Watts
Receiver Gain:	36
Offset Frequency:	3290.61 Hz
Presaturation Power Level:	0.0000964 Watts
Chemical Shift Ref Cpd:	DSS-d6
Temperature:	25 C
Number Of Scans:	64
Dummy Scans:	4
Acquisition Time:	3.9 seconds
Relaxation Delay:	2 seconds
Spectral Width:	12 ppm
Num Data Points Acquired:	65536
Real Data Points:	32768
Line Broadening:	0.5 Hz
Zero Filling:	Yes
Apodization:	Lorentzian
Baseline Correction Method:	Polynomial
Chemical Shift Ref Std:	DSS-d6
Binned Increment:	0.04ppm
Binned Data Excluded Range:	4.79 - 4.85 ppm (Water region)