Signal intensities derived from different NMR probes and parameters contribute to variations in quantification of metabolites.
We discovered that serious issues could arise that may complicate interpretation of metabolomic data when identical samples are analyzed at more than one NMR facility, or using slightly different NMR parameters on the same instrument. This is important because cross-center validation metabolomics st...
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doaj-4d2822456dfa4df7a5a265b492cf18332020-11-25T01:00:25ZengPublic Library of Science (PLoS)PLoS ONE1932-62032014-01-0191e8573210.1371/journal.pone.0085732Signal intensities derived from different NMR probes and parameters contribute to variations in quantification of metabolites.Paige LacyRyan T McKayMichael FinkelAlla KarnovskyScott WoehlerMichael J LewisDavid ChangKathleen A StringerWe discovered that serious issues could arise that may complicate interpretation of metabolomic data when identical samples are analyzed at more than one NMR facility, or using slightly different NMR parameters on the same instrument. This is important because cross-center validation metabolomics studies are essential for the reliable application of metabolomics to clinical biomarker discovery. To test the reproducibility of quantified metabolite data at multiple sites, technical replicates of urine samples were assayed by 1D-(1)H-NMR at the University of Alberta and the University of Michigan. Urine samples were obtained from healthy controls under a standard operating procedure for collection and processing. Subsequent analysis using standard statistical techniques revealed that quantitative data across sites can be achieved, but also that previously unrecognized NMR parameter differences can dramatically and widely perturb results. We present here a confirmed validation of NMR analysis at two sites, and report the range and magnitude that common NMR parameters involved in solvent suppression can have on quantitated metabolomics data. Specifically, saturation power levels greatly influenced peak height intensities in a frequency-dependent manner for a number of metabolites, which markedly impacted the quantification of metabolites. We also investigated other NMR parameters to determine their effects on further quantitative accuracy and precision. Collectively, these findings highlight the importance of and need for consistent use of NMR parameter settings within and across centers in order to generate reliable, reproducible quantified NMR metabolomics data.http://europepmc.org/articles/PMC3897511?pdf=render |
collection |
DOAJ |
language |
English |
format |
Article |
sources |
DOAJ |
author |
Paige Lacy Ryan T McKay Michael Finkel Alla Karnovsky Scott Woehler Michael J Lewis David Chang Kathleen A Stringer |
spellingShingle |
Paige Lacy Ryan T McKay Michael Finkel Alla Karnovsky Scott Woehler Michael J Lewis David Chang Kathleen A Stringer Signal intensities derived from different NMR probes and parameters contribute to variations in quantification of metabolites. PLoS ONE |
author_facet |
Paige Lacy Ryan T McKay Michael Finkel Alla Karnovsky Scott Woehler Michael J Lewis David Chang Kathleen A Stringer |
author_sort |
Paige Lacy |
title |
Signal intensities derived from different NMR probes and parameters contribute to variations in quantification of metabolites. |
title_short |
Signal intensities derived from different NMR probes and parameters contribute to variations in quantification of metabolites. |
title_full |
Signal intensities derived from different NMR probes and parameters contribute to variations in quantification of metabolites. |
title_fullStr |
Signal intensities derived from different NMR probes and parameters contribute to variations in quantification of metabolites. |
title_full_unstemmed |
Signal intensities derived from different NMR probes and parameters contribute to variations in quantification of metabolites. |
title_sort |
signal intensities derived from different nmr probes and parameters contribute to variations in quantification of metabolites. |
publisher |
Public Library of Science (PLoS) |
series |
PLoS ONE |
issn |
1932-6203 |
publishDate |
2014-01-01 |
description |
We discovered that serious issues could arise that may complicate interpretation of metabolomic data when identical samples are analyzed at more than one NMR facility, or using slightly different NMR parameters on the same instrument. This is important because cross-center validation metabolomics studies are essential for the reliable application of metabolomics to clinical biomarker discovery. To test the reproducibility of quantified metabolite data at multiple sites, technical replicates of urine samples were assayed by 1D-(1)H-NMR at the University of Alberta and the University of Michigan. Urine samples were obtained from healthy controls under a standard operating procedure for collection and processing. Subsequent analysis using standard statistical techniques revealed that quantitative data across sites can be achieved, but also that previously unrecognized NMR parameter differences can dramatically and widely perturb results. We present here a confirmed validation of NMR analysis at two sites, and report the range and magnitude that common NMR parameters involved in solvent suppression can have on quantitated metabolomics data. Specifically, saturation power levels greatly influenced peak height intensities in a frequency-dependent manner for a number of metabolites, which markedly impacted the quantification of metabolites. We also investigated other NMR parameters to determine their effects on further quantitative accuracy and precision. Collectively, these findings highlight the importance of and need for consistent use of NMR parameter settings within and across centers in order to generate reliable, reproducible quantified NMR metabolomics data. |
url |
http://europepmc.org/articles/PMC3897511?pdf=render |
work_keys_str_mv |
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