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Yeast Carbon Catabolite Repression

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TLDR
It is possible in certain cases to propose a partial model of the way in which the different elements involved in catabolite repression may be integrated, and preliminary evidence suggests that Snf1 is in a dephosphorylated state under these conditions.
Abstract
Glucose and related sugars repress the transcription of genes encoding enzymes required for the utilization of alternative carbon sources; some of these genes are also repressed by other sugars such as galactose, and the process is known as catabolite repression. The different sugars produce signals which modify the conformation of certain proteins that, in turn, directly or through a regulatory cascade affect the expression of the genes subject to catabolite repression. These genes are not all controlled by a single set of regulatory proteins, but there are different circuits of repression for different groups of genes. However, the protein kinase Snf1/Cat1 is shared by the various circuits and is therefore a central element in the regulatory process. Snf1 is not operative in the presence of glucose, and preliminary evidence suggests that Snf1 is in a dephosphorylated state under these conditions. However, the enzymes that phosphorylate and dephosphorylate Snf1 have not been identified, and it is not known how the presence of glucose may affect their activity. What has been established is that Snf1 remains active in mutants lacking either the proteins Grr1/Cat80 or Hxk2 or the Glc7 complex, which functions as a protein phosphatase. One of the main roles of Snf1 is to relieve repression by the Mig1 complex, but it is also required for the operation of transcription factors such as Adr1 and possibly other factors that are still unidentified. Although our knowledge of catabolite repression is still very incomplete, it is possible in certain cases to propose a partial model of the way in which the different elements involved in catabolite repression may be integrated.

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References
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Journal ArticleDOI

Derepression of Gene Expression Mediated by the 5′ Upstream Region of the Isocitrate Lyase Gene of Candida Tropicalis is Controlled by two Distinct Regulatory Pathways in Saccharomyces Cerevisiae

TL;DR: Investigation of regions in UPR-ICL responsible for gene expression in glucose-grown and acetate-grown cells indicates that region-A1-mediated gene expression is regulated by a pathway independent of CAT8, which is necessary for derepression of CSRE-mediated genes expression in S. cerevisiae.
Journal ArticleDOI

Functional analysis of upstream activating elements in the promoter of the FBP1 gene from Saccharomyces cerevisiae

TL;DR: In vivo the operation of both UASs is high in ethanol, moderate to low in glycerol, and negligible in galactose, and there is no effect of a MIG1 deletion, either in the formation of DNA-protein complexes or on the expression of reporter genes.
Journal ArticleDOI

Isolation and identification of genes activating UAS2-dependent ADH2 expression in Saccharomyces cerevisiae.

TL;DR: Two cis-acting elements have been identified that act synergistically to regulate expression of the glucose-repressed alcohol dehydrogenase 2 (ADH2) gene.
Journal ArticleDOI

Parallel changes in catabolite repression of haem biosynthesis and cytochromes in repression-resistant mutants of Saccharomyces cerevisiae.

TL;DR: Co-inheritance of the latter traits, sensitivity to maltose inhibition and ability to grow on raffinose in the presence of 2-deoxyglucose, demonstrated that the pleiotropic phenotype is a function of the single gene hex2-3.
Journal ArticleDOI

The 15 N-terminal amino acids of hexokinase II are not required for in vivo function: analysis of a truncated form of hexokinase II in Saccharomyces cerevisiae.

TL;DR: It is concluded that the N‐terminalamino acids of hexokinase II are not required in vivo either for phosporylation of hexoses or for glucose repression.
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