Transcriptome analysis of a respiratory Saccharomycescerevisiae strain suggests the expression of its phenotype is glucose insensitive and predominantly controlled by Hap4, Cat8 and MigI
Artikel i vetenskaplig tidskrift, 2008

Background: We previously described the first respiratory Saccharomyces cerevisiae strain, KOY.TM6*P, by integrating the gene encoding a chimeric hexose transporter, Tm6*, into the genome of an hxt null yeast. Subsequently we transferred this respiratory phenotype in the presence of up to 50 g/L glucose to a yeast strain, V5 hxt1-7Δ, in which only HXT1-7 had been deleted. In this study, we compared the transcriptome of the resultant strain, V5.TM*P, with that of its wild-type parent, V5, at different glucose concentrations. Results: cDNA array analyses revealed that alterations in gene expression that occur when transitioning from a respiro-fermentative (V5) to a respiratory (V5.TM6*P) strain, are very similar to those in cells undergoing a diauxic shift. We also undertook an analysis of transcription factor binding sites in our dataset by examining previously-published biological data for Hap4 (in complex with Hap2, 3, 5), Cat8 and Mig1, and used this in combination with verified binding consensus sequences to identify genes likely to be regulated by one or more of these. Of the induced genes in our dataset, 77% had binding sites for the Hap complex, with 72% having at least two. In addition, 13% were found to have a binding site for Cat8 and 21% had a binding site for Mig1. Unexpectedly, both the up- and down-regulation of many of the genes in our dataset had a clear glucose dependence in the parent V5 strain that was not present in V5.TM6*P. This indicates that the relief of glucose repression is already operable at much higher glucose concentrations than is widely accepted and suggests that glucose sensing might occur inside the cell. Conclusion: Our dataset gives a remarkably complete view of the involvement of genes in the TCA cycle, glyoxylate cycle and respiratory chain in the expression of the phenotype of V5.TM6*P. Furthermore, 88% of the transcriptional response of the induced genes in our dataset can be related to the potential activities of just three proteins: Hap4, Cat8 and Mig1. Overall, our data support genetic remodelling in V5.TM6*P consistent with a respiratory metabolism which is insensitive to external glucose concentrations. © 2008 Bonander et al; licensee BioMed Central Ltd.

yeast

cerevisiae

chemostat cultures

carbon metabolism

genes

protein

binding

glycolytic-enzymes

overexpression

messenger-rnas

Författare

Nicklas Bonander

Aston University

Cecilia Ferndahl

Chalmers, Kemi- och bioteknik, Molekylär mikroskopi

Petter Mostad

Göteborgs universitet

Chalmers, Matematiska vetenskaper, matematisk statistik

Martin D. B. Wilks

Cameron International Ltd

Celia Chang

The Wistar Institute

Louise Showe

The Wistar Institute

Lena Gustafsson

Chalmers, Kemi- och bioteknik, Molekylär mikroskopi

Christer Larsson

Chalmers, Kemi- och bioteknik, Molekylär mikroskopi

R Bill

Aston University

BMC Genomics

1471-2164 (ISSN)

Vol. 9 365-

Ämneskategorier

Industriell bioteknik

Genetik

DOI

10.1186/1471-2164-9-365

Mer information

Skapat

2017-10-07