Abstract

The goals of this research plan are to elucidate the mechanisms involved in regulating transcription of glycolytic and ribosomal RNA genes in Saccharomyces cerevisiae. Distinct cis-acting sequences which mediate positive or negative regulation of transcription of the two enolase genes (ENO1 and ENO2) and one of the glyceraldehyde-3-phosphate dehydrogenase genes (TDH3) have been mapped within the 5' flanking regions of each gene. Proteins which form stable complexes with these cis-acting regulatory sequences have been identified using DNA/protein binding assays. Genetic and biochemical studies suggest that the GCR1 gene product, which is required for efficient transcription of most glycolytic genes, interferes with the binding of a repressor-like protein to a site within the upstream activation sequences (UAS) of ENO2. The GCR1 protein and the repressor protein will be purified and extensively characterized with respect to their roles in coordinate regulation of ENO1, ENO2, and TDH3 expression. Mutant strains which are defective in the repressor gene will be isolated and characterized. Utilizing these mutant strains and the purified regulatory proteins, correlations will be made between specific DNA/protein binding events and expression of the glycolytic gene under study in cells grown on glycolytic or gluconeogenic carbon soruces. A protein which binds to the upstream repression sequences (URS) in ENO1 will also be purified. The effects of the URS binding protein on the binding of other regulatory proteins to the ENO1 UAS regions or TATAAA sequences will be investigated. Mutant strains which are defective in the URS binding protein gene will be isolated and characterized. A highly sensitive assay for detecting RNA polymerase II-dependent selective initiation of transcription in vitro will be developed. Once an in vitro transcription assay is available, it will be used in conjunction with the aforementioned binding studies and genetic analyses to further elucidate the mechanisms involved in regulating glycolytic gene expression. The sequence requirements for synthesis of 34SrRNA in vivo will be further defined using a centromere plasmid carrying an artificial 35SrRNA gene. These studies will be aimed toward establishing the transcriptional function of sequences adjacent to the 34SrRNA initiation site in the presence and absence of a spacer promoter sequence which stimulates 35SrRNA synthesis in vivo more than 10-fold. Factors required for RNA polymerase I- dependent selective transcription from the spacer promoter will be purified and used to reconstitute accurate transcription in vitro.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
2R01GM030307-07
Application #
3277957
Study Section
Genetics Study Section (GEN)
Project Start
1981-05-01
Project End
1992-04-30
Budget Start
1987-05-01
Budget End
1988-04-30
Support Year
7
Fiscal Year
1987
Total Cost
Indirect Cost

  Institution

Name
University of California Davis
Department
Type
Schools of Medicine
DUNS #
094878337
City
Davis
State
CA
Country
United States
Zip Code
95618

  Publications

Nishi, K; Park, C S; Pepper, A E et al. (1995) The GCR1 requirement for yeast glycolytic gene expression is suppressed by dominant mutations in the SGC1 gene, which encodes a novel basic-helix-loop-helix protein. Mol Cell Biol 15:2646-53
Kang, J J; Yokoi, T J; Holland, M J (1995) Binding sites for abundant nuclear factors modulate RNA polymerase I-dependent enhancer function in Saccharomyces cerevisiae. J Biol Chem 270:28723-32
Carmen, A A; Holland, M J (1994) The upstream repression sequence from the yeast enolase gene ENO1 is a complex regulatory element that binds multiple trans-acting factors including REB1. J Biol Chem 269:9790-7
Willett, C E; Gelfman, C M; Holland, M J (1993) A complex regulatory element from the yeast gene ENO2 modulates GCR1-dependent transcriptional activation. Mol Cell Biol 13:2623-33
Holland, J P; Brindle, P K; Holland, M J (1990) Sequences within an upstream activation site in the yeast enolase gene ENO2 modulate repression of ENO2 expression in strains carrying a null mutation in the positive regulatory gene GCR1. Mol Cell Biol 10:4863-71
Brindle, P K; Holland, J P; Willett, C E et al. (1990) Multiple factors bind the upstream activation sites of the yeast enolase genes ENO1 and ENO2: ABFI protein, like repressor activator protein RAP1, binds cis-acting sequences which modulate repression or activation of transcription. Mol Cell Biol 10:4872-85
Yip, M T; Holland, M J (1989) In vitro RNA processing generates mature 3' termini of yeast 35 and 25 S ribosomal RNAs. J Biol Chem 264:4045-51
Mestel, R; Yip, M; Holland, J P et al. (1989) Sequences within the spacer region of yeast rRNA cistrons that stimulate 35S rRNA synthesis in vivo mediate RNA polymerase I-dependent promoter and terminator activities. Mol Cell Biol 9:1243-54
Holland, M J; Yokoi, T; Holland, J P et al. (1987) The GCR1 gene encodes a positive transcriptional regulator of the enolase and glyceraldehyde-3-phosphate dehydrogenase gene families in Saccharomyces cerevisiae. Mol Cell Biol 7:813-20
Cohen, R; Yokoi, T; Holland, J P et al. (1987) Transcription of the constitutively expressed yeast enolase gene ENO1 is mediated by positive and negative cis-acting regulatory sequences. Mol Cell Biol 7:2753-61

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