Literature DB >> 27572163

The metabolic background is a global player in Saccharomyces gene expression epistasis.

Mohammad Tauqeer Alam1, Aleksej Zelezniak1,2, Michael Mülleder1, Pavel Shliaha1,3, Roland Schwarz4, Floriana Capuano1, Jakob Vowinckel1, Elahe Radmanesfahar1, Antje Krüger5, Enrica Calvani1, Steve Michel5, Stefan Börno5, Stefan Christen6, Kiran Raosaheb Patil7, Bernd Timmermann5, Kathryn S Lilley1,3, Markus Ralser1,2.   

Abstract

The regulation of gene expression in response to nutrient availability is fundamental to the genotype-phenotype relationship. The metabolic-genetic make-up of the cell, as reflected in auxotrophy, is hence likely to be a determinant of gene expression. Here, we address the importance of the metabolic-genetic background by monitoring transcriptome, proteome and metabolome in a repertoire of 16 Saccharomyces cerevisiae laboratory backgrounds, combinatorially perturbed in histidine, leucine, methionine and uracil biosynthesis. The metabolic background affected up to 85% of the coding genome. Suggesting widespread confounding, these transcriptional changes show, on average, 83% overlap between unrelated auxotrophs and 35% with previously published transcriptomes generated for non-metabolic gene knockouts. Background-dependent gene expression correlated with metabolic flux and acted, predominantly through masking or suppression, on 88% of transcriptional interactions epistatically. As a consequence, the deletion of the same metabolic gene in a different background could provoke an entirely different transcriptional response. Propagating to the proteome and scaling up at the metabolome, metabolic background dependencies reveal the prevalence of metabolism-dependent epistasis at all regulatory levels. Urging a fundamental change of the prevailing laboratory practice of using auxotrophs and nutrient supplemented media, these results reveal epistatic intertwining of metabolism with gene expression on the genomic scale.

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Year:  2016        PMID: 27572163      PMCID: PMC5131842          DOI: 10.1038/nmicrobiol.2015.30

Source DB:  PubMed          Journal:  Nat Microbiol        ISSN: 2058-5276            Impact factor:   17.745


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