Functional characterization of transcriptional regulatory elements in the upstream region of the yeast GLK1 gene

P Herrero; L Flores; T de la Cera; F Moreno

Functional characterization of transcriptional regulatory elements in the upstream region of the yeast GLK1 gene

Biochem J. 1999 Oct 15;343 Pt 2(Pt 2):319-25.

Authors

P Herrero¹, L Flores, T de la Cera, F Moreno

Affiliation

¹ Departamento de Bioqu approximately ímica y Biolog approximately ía Molecular, Instituto Universitario de Biotecnolog approximately ía de Asturias, Universidad de Oviedo, 33006 Oviedo, Spain.

PMID: 10510295
PMCID: PMC1220556

Abstract

The glucokinase gene GLK1 of the yeast Saccharomyces cerevisiae is transcriptionally regulated in response to the carbon source of the growth medium. Northern-blot analysis shows that the GLK1 gene is expressed at a basal level in the presence of glucose, de-repressed more than 6-fold under conditions of sugar limitation and more than 25-fold under conditions of ethanol induction. lacZ fusions of the GLK1 gene promoter were constructed and a deletion analysis was performed in order to identify the cis-acting regulatory elements of the promoter that controls GLK1 gene expression. First, the expression seemed to be mediated mainly by one GCR1 and three stress-responsive element (STRE) activating elements. Secondly, an ethanol repression autoregulation (ERA)/twelve-fold TA repeat (TAB) repressor element was identified within the promoter region of the GLK1 gene. A specific and differential protein binding to the STRE was observed with extracts from de-repressed and repressed cells. No differential binding to the GCR1 or ERA/TAB elements was observed with extracts from de-repressed and repressed cells, but, in both cases, the binding was competed for by an excess of the unlabelled GLK1(GCR1) and GLK1(ERA) sequence. The transcription factors Msn2 and Msn4, which bind to the GLK1 upstream region through the STRE, contribute to inductive activation. The transcription factor Gcr1, which binds through the GCR1 element, contributes to constitutive activation. In order to achieve the severe glucose repression of GLK1, constitutive repressor factors acting through the ERA/TAB element must counteract constitutive activation generated by Gcr1 binding to the GCR1 element. Full expression of the GLK1 gene is produced by inductive activation of three STRE when Msn2 and Msn4 proteins are translocated to the nucleus by covalent modification. The combinatorial effect of the entire region leads to the regulated transcription of GLK1, i.e., silent in media with glucose and other preferred carbon sources, such as fructose or mannose, and increased levels of expression upon glucose depletion.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Base Sequence
Binding Sites
Carbon / metabolism
DNA / genetics
DNA / metabolism
DNA-Binding Proteins / metabolism
Ethanol / metabolism
Ethanol / pharmacology
Fungal Proteins / metabolism
Gene Expression Regulation, Fungal* / drug effects
Glucokinase / genetics*
Glucose / metabolism
Promoter Regions, Genetic / genetics
RNA, Messenger / genetics
RNA, Messenger / metabolism
Repressor Proteins / metabolism
Response Elements / genetics*
Saccharomyces cerevisiae / drug effects
Saccharomyces cerevisiae / enzymology*
Saccharomyces cerevisiae / genetics*
Saccharomyces cerevisiae / metabolism
Saccharomyces cerevisiae Proteins*
Sequence Deletion
Transcription Factors / metabolism

Substances

DNA-Binding Proteins
Fungal Proteins
MSN2 protein, S cerevisiae
MSN4 protein, S cerevisiae
RNA, Messenger
Repressor Proteins
Saccharomyces cerevisiae Proteins
Transcription Factors
Ethanol
Carbon
DNA
Glucokinase
Glucose