High-Performance Chemical Isotope Labeling Liquid Chromatography–Mass Spectrometry for Profiling the Metabolomic Reprogramming Elicited by Ammonium Limitation in Yeast

High-Performance Chemical Isotope Labeling Liquid Chromatography–Mass Spectrometry for Profiling the Metabolomic Reprogramming Elicited by Ammonium Limitation in Yeast

Information about how yeast metabolism is rewired in response to internal and external cues can inform the development of metabolic engineering strategies for food, fuel, and chemical production in this organism. We report a new metabolomics workflow for the characterization of such metabolic rewiri...

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Veröffentlicht in:Journal of proteome research 2016-05, Vol.15 (5), p.1602-1612
Hauptverfasser: Luo, Xian, Zhao, Shuang, Huan, Tao, Sun, Difei, Friis, R. Magnus N, Schultz, Michael C, Li, Liang
Format: Artikel
Sprache:eng
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Acetyl Coenzyme A - biosynthesis
Amines - metabolism
Ammonium Compounds - metabolism
Carboxylic Acids - metabolism
Chromatography, Liquid - methods
Data Mining
Isotope Labeling
Mass Spectrometry - methods
Metabolic Engineering - methods
Metabolomics - methods
Phenols - metabolism
Saccharomyces cerevisiae - metabolism
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container_end_page 1612
container_issue 5
container_start_page 1602
container_title Journal of proteome research
container_volume 15
creator Luo, Xian
Zhao, Shuang
Huan, Tao
Sun, Difei
Friis, R. Magnus N
Schultz, Michael C
Li, Liang
description Information about how yeast metabolism is rewired in response to internal and external cues can inform the development of metabolic engineering strategies for food, fuel, and chemical production in this organism. We report a new metabolomics workflow for the characterization of such metabolic rewiring. The workflow combines efficient cell lysis without using chemicals that may interfere with downstream sample analysis and differential chemical isotope labeling liquid chromatography mass spectrometry (CIL LC–MS) for in-depth yeast metabolome profiling. Using 12C- and 13C-dansylation (Dns) labeling to analyze the amine/phenol submetabolome, we detected and quantified a total of 5719 peak pairs or metabolites. Among them, 120 metabolites were positively identified using a library of 275 Dns-metabolite standards, and 2980 metabolites were putatively identified based on accurate mass matches to metabolome databases. We also applied 12C- and 13C-dimethylaminophenacyl (DmPA) labeling to profile the carboxylic acid submetabolome and detected over 2286 peak pairs, from which 33 metabolites were positively identified using a library of 188 DmPA-metabolite standards, and 1595 metabolites were putatively identified. Using this workflow for metabolomic profiling of cells challenged by ammonium limitation revealed unexpected links between ammonium assimilation and pantothenate accumulation that might be amenable to engineering for better acetyl-CoA production in yeast. We anticipate that efforts to improve other schemes of metabolic engineering will benefit from application of this workflow to multiple cell types.
doi_str_mv 10.1021/acs.jproteome.6b00070
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subjects Acetyl Coenzyme A - biosynthesis
Amines - metabolism
Ammonium Compounds - metabolism
Carboxylic Acids - metabolism
Chromatography, Liquid - methods
Data Mining
Isotope Labeling
Mass Spectrometry - methods
Metabolic Engineering - methods
Metabolomics - methods
Phenols - metabolism
Saccharomyces cerevisiae - metabolism
title High-Performance Chemical Isotope Labeling Liquid Chromatography–Mass Spectrometry for Profiling the Metabolomic Reprogramming Elicited by Ammonium Limitation in Yeast
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