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A novel stable isotope labelling assisted workflow for improved untargeted LC–HRMS based metabolomics research

Many untargeted LC–ESI–HRMS based metabolomics studies are still hampered by the large proportion of non-biological sample derived signals included in the generated raw data. Here, a novel, powerful stable isotope labelling (SIL)-based metabolomics workflow is presented, which facilitates global met...

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Autores principales: Bueschl, Christoph, Kluger, Bernhard, Lemmens, Marc, Adam, Gerhard, Wiesenberger, Gerlinde, Maschietto, Valentina, Marocco, Adriano, Strauss, Joseph, Bödi, Stephan, Thallinger, Gerhard G., Krska, Rudolf, Schuhmacher, Rainer
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Springer US 2013
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4098048/
https://www.ncbi.nlm.nih.gov/pubmed/25057268
http://dx.doi.org/10.1007/s11306-013-0611-0
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author Bueschl, Christoph
Kluger, Bernhard
Lemmens, Marc
Adam, Gerhard
Wiesenberger, Gerlinde
Maschietto, Valentina
Marocco, Adriano
Strauss, Joseph
Bödi, Stephan
Thallinger, Gerhard G.
Krska, Rudolf
Schuhmacher, Rainer
author_facet Bueschl, Christoph
Kluger, Bernhard
Lemmens, Marc
Adam, Gerhard
Wiesenberger, Gerlinde
Maschietto, Valentina
Marocco, Adriano
Strauss, Joseph
Bödi, Stephan
Thallinger, Gerhard G.
Krska, Rudolf
Schuhmacher, Rainer
author_sort Bueschl, Christoph
collection PubMed
description Many untargeted LC–ESI–HRMS based metabolomics studies are still hampered by the large proportion of non-biological sample derived signals included in the generated raw data. Here, a novel, powerful stable isotope labelling (SIL)-based metabolomics workflow is presented, which facilitates global metabolome extraction, improved metabolite annotation and metabolome wide internal standardisation (IS). The general concept is exemplified with two different cultivation variants, (1) co-cultivation of the plant pathogenic fungi Fusarium graminearum on non-labelled and highly (13)C enriched culture medium and (2) experimental cultivation under native conditions and use of globally U-(13)C labelled biological reference samples as exemplified with maize and wheat. Subsequent to LC–HRMS analysis of mixtures of labelled and non-labelled samples, two-dimensional data filtering of SIL specific isotopic patterns is performed to better extract truly biological derived signals together with the corresponding number of carbon atoms of each metabolite ion. Finally, feature pairs are convoluted to feature groups each representing a single metabolite. Moreover, the correction of unequal matrix effects in different sample types and the improvement of relative metabolite quantification with metabolome wide IS are demonstrated for the F. graminearum experiment. Data processing employing the presented workflow revealed about 300 SIL derived feature pairs corresponding to 87–135 metabolites in F. graminearum samples and around 800 feature pairs corresponding to roughly 350 metabolites in wheat samples. SIL assisted IS, by the use of globally U-(13)C labelled biological samples, reduced the median CV value from 7.1 to 3.6 % for technical replicates and from 15.1 to 10.8 % for biological replicates in the respective F. graminearum samples.
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spelling pubmed-40980482014-07-21 A novel stable isotope labelling assisted workflow for improved untargeted LC–HRMS based metabolomics research Bueschl, Christoph Kluger, Bernhard Lemmens, Marc Adam, Gerhard Wiesenberger, Gerlinde Maschietto, Valentina Marocco, Adriano Strauss, Joseph Bödi, Stephan Thallinger, Gerhard G. Krska, Rudolf Schuhmacher, Rainer Metabolomics Original Article Many untargeted LC–ESI–HRMS based metabolomics studies are still hampered by the large proportion of non-biological sample derived signals included in the generated raw data. Here, a novel, powerful stable isotope labelling (SIL)-based metabolomics workflow is presented, which facilitates global metabolome extraction, improved metabolite annotation and metabolome wide internal standardisation (IS). The general concept is exemplified with two different cultivation variants, (1) co-cultivation of the plant pathogenic fungi Fusarium graminearum on non-labelled and highly (13)C enriched culture medium and (2) experimental cultivation under native conditions and use of globally U-(13)C labelled biological reference samples as exemplified with maize and wheat. Subsequent to LC–HRMS analysis of mixtures of labelled and non-labelled samples, two-dimensional data filtering of SIL specific isotopic patterns is performed to better extract truly biological derived signals together with the corresponding number of carbon atoms of each metabolite ion. Finally, feature pairs are convoluted to feature groups each representing a single metabolite. Moreover, the correction of unequal matrix effects in different sample types and the improvement of relative metabolite quantification with metabolome wide IS are demonstrated for the F. graminearum experiment. Data processing employing the presented workflow revealed about 300 SIL derived feature pairs corresponding to 87–135 metabolites in F. graminearum samples and around 800 feature pairs corresponding to roughly 350 metabolites in wheat samples. SIL assisted IS, by the use of globally U-(13)C labelled biological samples, reduced the median CV value from 7.1 to 3.6 % for technical replicates and from 15.1 to 10.8 % for biological replicates in the respective F. graminearum samples. Springer US 2013-12-04 2014 /pmc/articles/PMC4098048/ /pubmed/25057268 http://dx.doi.org/10.1007/s11306-013-0611-0 Text en © The Author(s) 2013 https://creativecommons.org/licenses/by/2.0/ Open AccessThis article is distributed under the terms of the Creative Commons Attribution License which permits any use, distribution, and reproduction in any medium, provided the original author(s) and the source are credited.
spellingShingle Original Article
Bueschl, Christoph
Kluger, Bernhard
Lemmens, Marc
Adam, Gerhard
Wiesenberger, Gerlinde
Maschietto, Valentina
Marocco, Adriano
Strauss, Joseph
Bödi, Stephan
Thallinger, Gerhard G.
Krska, Rudolf
Schuhmacher, Rainer
A novel stable isotope labelling assisted workflow for improved untargeted LC–HRMS based metabolomics research
title A novel stable isotope labelling assisted workflow for improved untargeted LC–HRMS based metabolomics research
title_full A novel stable isotope labelling assisted workflow for improved untargeted LC–HRMS based metabolomics research
title_fullStr A novel stable isotope labelling assisted workflow for improved untargeted LC–HRMS based metabolomics research
title_full_unstemmed A novel stable isotope labelling assisted workflow for improved untargeted LC–HRMS based metabolomics research
title_short A novel stable isotope labelling assisted workflow for improved untargeted LC–HRMS based metabolomics research
title_sort novel stable isotope labelling assisted workflow for improved untargeted lc–hrms based metabolomics research
topic Original Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4098048/
https://www.ncbi.nlm.nih.gov/pubmed/25057268
http://dx.doi.org/10.1007/s11306-013-0611-0
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