Metabolomics Data Normalization with EigenMS

Liquid chromatography mass spectrometry has become one of the analytical platforms of choice for metabolomics studies. However, LC-MS metabolomics data can suffer from the effects of various systematic biases. These include batch effects, day-to-day variations in instrument performance, signal inten...

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Published inPloS one Vol. 9; no. 12; p. e116221
Main Authors Karpievitch, Yuliya V., Nikolic, Sonja B., Wilson, Richard, Sharman, James E., Edwards, Lindsay M.
Format Journal Article
LanguageEnglish
Published United States Public Library of Science 30.12.2014
Public Library of Science (PLoS)
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Online AccessGet full text
ISSN1932-6203
1932-6203
DOI10.1371/journal.pone.0116221

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Abstract Liquid chromatography mass spectrometry has become one of the analytical platforms of choice for metabolomics studies. However, LC-MS metabolomics data can suffer from the effects of various systematic biases. These include batch effects, day-to-day variations in instrument performance, signal intensity loss due to time-dependent effects of the LC column performance, accumulation of contaminants in the MS ion source and MS sensitivity among others. In this study we aimed to test a singular value decomposition-based method, called EigenMS, for normalization of metabolomics data. We analyzed a clinical human dataset where LC-MS serum metabolomics data and physiological measurements were collected from thirty nine healthy subjects and forty with type 2 diabetes and applied EigenMS to detect and correct for any systematic bias. EigenMS works in several stages. First, EigenMS preserves the treatment group differences in the metabolomics data by estimating treatment effects with an ANOVA model (multiple fixed effects can be estimated). Singular value decomposition of the residuals matrix is then used to determine bias trends in the data. The number of bias trends is then estimated via a permutation test and the effects of the bias trends are eliminated. EigenMS removed bias of unknown complexity from the LC-MS metabolomics data, allowing for increased sensitivity in differential analysis. Moreover, normalized samples better correlated with both other normalized samples and corresponding physiological data, such as blood glucose level, glycated haemoglobin, exercise central augmentation pressure normalized to heart rate of 75, and total cholesterol. We were able to report 2578 discriminatory metabolite peaks in the normalized data (p<0.05) as compared to only 1840 metabolite signals in the raw data. Our results support the use of singular value decomposition-based normalization for metabolomics data.
AbstractList Liquid chromatography mass spectrometry has become one of the analytical platforms of choice for metabolomics studies. However, LC-MS metabolomics data can suffer from the effects of various systematic biases. These include batch effects, day-to-day variations in instrument performance, signal intensity loss due to time-dependent effects of the LC column performance, accumulation of contaminants in the MS ion source and MS sensitivity among others. In this study we aimed to test a singular value decomposition-based method, called EigenMS, for normalization of metabolomics data. We analyzed a clinical human dataset where LC-MS serum metabolomics data and physiological measurements were collected from thirty nine healthy subjects and forty with type 2 diabetes and applied EigenMS to detect and correct for any systematic bias. EigenMS works in several stages. First, EigenMS preserves the treatment group differences in the metabolomics data by estimating treatment effects with an ANOVA model (multiple fixed effects can be estimated). Singular value decomposition of the residuals matrix is then used to determine bias trends in the data. The number of bias trends is then estimated via a permutation test and the effects of the bias trends are eliminated. EigenMS removed bias of unknown complexity from the LC-MS metabolomics data, allowing for increased sensitivity in differential analysis. Moreover, normalized samples better correlated with both other normalized samples and corresponding physiological data, such as blood glucose level, glycated haemoglobin, exercise central augmentation pressure normalized to heart rate of 75, and total cholesterol. We were able to report 2578 discriminatory metabolite peaks in the normalized data (p<0.05) as compared to only 1840 metabolite signals in the raw data. Our results support the use of singular value decomposition-based normalization for metabolomics data.
Liquid chromatography mass spectrometry has become one of the analytical platforms of choice for metabolomics studies. However, LC-MS metabolomics data can suffer from the effects of various systematic biases. These include batch effects, day-to-day variations in instrument performance, signal intensity loss due to time-dependent effects of the LC column performance, accumulation of contaminants in the MS ion source and MS sensitivity among others. In this study we aimed to test a singular value decomposition-based method, called EigenMS, for normalization of metabolomics data. We analyzed a clinical human dataset where LC-MS serum metabolomics data and physiological measurements were collected from thirty nine healthy subjects and forty with type 2 diabetes and applied EigenMS to detect and correct for any systematic bias. EigenMS works in several stages. First, EigenMS preserves the treatment group differences in the metabolomics data by estimating treatment effects with an ANOVA model (multiple fixed effects can be estimated). Singular value decomposition of the residuals matrix is then used to determine bias trends in the data. The number of bias trends is then estimated via a permutation test and the effects of the bias trends are eliminated. EigenMS removed bias of unknown complexity from the LC-MS metabolomics data, allowing for increased sensitivity in differential analysis. Moreover, normalized samples better correlated with both other normalized samples and corresponding physiological data, such as blood glucose level, glycated haemoglobin, exercise central augmentation pressure normalized to heart rate of 75, and total cholesterol. We were able to report 2578 discriminatory metabolite peaks in the normalized data (p<0.05) as compared to only 1840 metabolite signals in the raw data. Our results support the use of singular value decomposition-based normalization for metabolomics data.Liquid chromatography mass spectrometry has become one of the analytical platforms of choice for metabolomics studies. However, LC-MS metabolomics data can suffer from the effects of various systematic biases. These include batch effects, day-to-day variations in instrument performance, signal intensity loss due to time-dependent effects of the LC column performance, accumulation of contaminants in the MS ion source and MS sensitivity among others. In this study we aimed to test a singular value decomposition-based method, called EigenMS, for normalization of metabolomics data. We analyzed a clinical human dataset where LC-MS serum metabolomics data and physiological measurements were collected from thirty nine healthy subjects and forty with type 2 diabetes and applied EigenMS to detect and correct for any systematic bias. EigenMS works in several stages. First, EigenMS preserves the treatment group differences in the metabolomics data by estimating treatment effects with an ANOVA model (multiple fixed effects can be estimated). Singular value decomposition of the residuals matrix is then used to determine bias trends in the data. The number of bias trends is then estimated via a permutation test and the effects of the bias trends are eliminated. EigenMS removed bias of unknown complexity from the LC-MS metabolomics data, allowing for increased sensitivity in differential analysis. Moreover, normalized samples better correlated with both other normalized samples and corresponding physiological data, such as blood glucose level, glycated haemoglobin, exercise central augmentation pressure normalized to heart rate of 75, and total cholesterol. We were able to report 2578 discriminatory metabolite peaks in the normalized data (p<0.05) as compared to only 1840 metabolite signals in the raw data. Our results support the use of singular value decomposition-based normalization for metabolomics data.
Audience Academic
Author Sharman, James E.
Nikolic, Sonja B.
Karpievitch, Yuliya V.
Edwards, Lindsay M.
Wilson, Richard
AuthorAffiliation 2 Menzies Research Institute Tasmania, University of Tasmania, Hobart, TAS, Australia
1 School of Mathematics and Physics, University of Tasmania, Hobart, TAS, Australia
4 Centre of Human & Aerospace Physiological Sciences, King’s College London, London, United Kingdom
3 Central Science Laboratory, University of Tasmania, Hobart, TAS, Australia
5 Fibrosis Discovery Performance Unit, GlaxoSmithKline R&D, Stevenage, United Kingdom
University of Westminster, United Kingdom
AuthorAffiliation_xml – name: 5 Fibrosis Discovery Performance Unit, GlaxoSmithKline R&D, Stevenage, United Kingdom
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– name: 2 Menzies Research Institute Tasmania, University of Tasmania, Hobart, TAS, Australia
– name: University of Westminster, United Kingdom
– name: 3 Central Science Laboratory, University of Tasmania, Hobart, TAS, Australia
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  givenname: Yuliya V.
  surname: Karpievitch
  fullname: Karpievitch, Yuliya V.
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  surname: Sharman
  fullname: Sharman, James E.
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  fullname: Edwards, Lindsay M.
BackLink https://www.ncbi.nlm.nih.gov/pubmed/25549083$$D View this record in MEDLINE/PubMed
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ContentType Journal Article
Copyright COPYRIGHT 2014 Public Library of Science
2014 Karpievitch et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License: http://creativecommons.org/licenses/by/4.0/ (the “License”), which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Notwithstanding the ProQuest Terms and Conditions, you may use this content in accordance with the terms of the License.
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Competing Interests: One of the authors is employed by a commercial company GlaxoSmithKline R&D. We note that this does not alter the authors’ adherence to PLOS ONE policies on sharing data and materials.
Conceived and designed the experiments: YVK SBN RW JES LME. Performed the experiments: SBN RW. Analyzed the data: YVK SBN LME. Contributed reagents/materials/analysis tools: YVK SBN RW JES LME. Contributed to the writing of the manuscript: YVK SBN RW JES LME.
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Snippet Liquid chromatography mass spectrometry has become one of the analytical platforms of choice for metabolomics studies. However, LC-MS metabolomics data can...
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SubjectTerms Aged
Bias
Biology and Life Sciences
Blood sugar
Cholesterol
Chromatography
Chromatography, Liquid - methods
Contaminants
Correlation analysis
Data processing
Databases, Factual
Decomposition
Diabetes
Diabetes mellitus
Diabetes mellitus (non-insulin dependent)
Diabetes Mellitus, Type 2 - blood
Diabetes Mellitus, Type 2 - metabolism
Experiments
Gene expression
Heart rate
Hemoglobin
Humans
Laboratories
Liquid chromatography
Mass spectrometry
Mass Spectrometry - methods
Mass spectroscopy
Metabolism
Metabolites
Metabolomics
Metabolomics - methods
Methods
Middle Aged
Permutations
Physical Sciences
Physiology
Proteomics
Reproducibility of Results
Research and Analysis Methods
Scientific imaging
Sensitivity
Sensitivity analysis
Singular value decomposition
Software
Studies
Time dependence
Trends
Urine
Variance analysis
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Title Metabolomics Data Normalization with EigenMS
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