Abstract

The mechanisms by which eukaryotic organisms regulate gene expression are important for basic scientific knowledge that is necessary for understanding many complex biological phenomena including human diseases. With regard to the process of transcriptional initiation, a wide variety of experiments have pointed to common molecular mechanisms in eukaryotic organisms ranging from humans to yeasts. Previous analysis of the yeast his3 gene has defined DNA sequences necessary for expression and regulation, has identified and characterized GCN4 protein, which is necessary for transcriptional activation, and has shown that expression is governed by two promoters that work by distinct molecular mechanisms. This proposal will investigate several basic issues concerning the molecular mechanisms involved in his3 transcriptional regulation by combining a wide variety of techniques including recombinant DNA technology, molecular and classical yeast genetics, and protein and nucleic acid biochemistry. First, the molecular basis for specific binding of GCN4 protein to the his3 regulatory site will be addressed by using degenerate oligonucleotides to create a large number of mutations within the DNA-binding domain of GCN4. The mutants will be examined in vivo and in vitro for DNA-binding, dimerization, alterations in DNA sequence recognition, and overall structure. Second, the critical features of the short acidic region of GCN4 required for transcriptional activation will be defined by deletion and point mutational analysis. Peptides containing a functional activation region will be synthesized and analyzed for effects on chromatin structure and for potential interactions with other proteins. Third, proteins interacting with GCN4 will be sought by biochemical approaches or by genetic selections to identify the the encoding genes. Biochemical approaches include affinity chromotography to GCN4 or the activation peptide and detection of GCN4 protein-DNA complexes with altered electrophoretic mobilities. Genetic approaches include revertants of gcn4 transcriptional activation mutants and a novel selection scheme involving recombinant DNA libraries in a protein fusion vector. The genes and the encoded proteins will be characterized by standard techniques of yeast molecular biology. Fourth, proteins interacting with either of the two functionally distinct his3 TATA elements will be sought by standard purification or by obtaining suppressor mutations that revert the transcriptional defects of TATA point mutations. The genes encoding these proteins will be cloned with the goal of elucidating their structure and function. Fifth, the molecular basis of constitutive his3 expression will be examined by varying the length and quality of the poly (dA-dT) sequence that serves as the upstream promoter element. The effects on transcription will be correlated with DNA bending and affects on chromatin structure. In summary, the proposed experiments should provide important information on basic questions such as the molecular nature of protein-DNA interactions in eukaryotic gene regulation, interactions between upstream activator proteins and the general transcription machinery, and the relationship of chromatin structure to gene expression.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
2R01GM030186-07
Application #
3277809
Study Section
Molecular Biology Study Section (MBY)
Project Start
1982-03-01
Project End
1993-02-28
Budget Start
1988-03-01
Budget End
1989-02-28
Support Year
7
Fiscal Year
1988
Total Cost
Indirect Cost

  Institution

Name
Harvard University
Department
Type
Schools of Medicine
DUNS #
082359691
City
Boston
State
MA
Country
United States
Zip Code
02115

  Publications

Moqtaderi, Zarmik; Geisberg, Joseph V; Struhl, Kevin (2018) Extensive Structural Differences of Closely Related 3' mRNA Isoforms: Links to Pab1 Binding and mRNA Stability. Mol Cell 72:849-861.e6
Jin, Yi; Eser, Umut; Struhl, Kevin et al. (2017) The Ground State and Evolution of Promoter Region Directionality. Cell 170:889-898.e10
Petrenko, Natalia; Jin, Yi; Wong, Koon Ho et al. (2017) Evidence that Mediator is essential for Pol II transcription, but is not a required component of the preinitiation complex in vivo. Elife 6:
Petrenko, Natalia; Jin, Yi; Wong, Koon Ho et al. (2016) Mediator Undergoes a Compositional Change during Transcriptional Activation. Mol Cell 64:443-454
Miotto, Benoit; Ji, Zhe; Struhl, Kevin (2016) Selectivity of ORC binding sites and the relation to replication timing, fragile sites, and deletions in cancers. Proc Natl Acad Sci U S A 113:E4810-9
Jin, Yi; Geisberg, Joseph V; Moqtaderi, Zarmik et al. (2015) Mapping 3' mRNA isoforms on a genomic scale. Curr Protoc Mol Biol 110:4.23.1-17
Wong, Koon Ho; Jin, Yi; Struhl, Kevin (2014) TFIIH phosphorylation of the Pol II CTD stimulates mediator dissociation from the preinitiation complex and promoter escape. Mol Cell 54:601-12
Moqtaderi, Zarmik; Geisberg, Joseph V; Struhl, Kevin (2014) Secondary structures involving the poly(A) tail and other 3' sequences are major determinants of mRNA isoform stability in yeast. Microb Cell 1:137-139
Geisberg, Joseph V; Moqtaderi, Zarmik; Fan, Xiaochun et al. (2014) Global analysis of mRNA isoform half-lives reveals stabilizing and destabilizing elements in yeast. Cell 156:812-24
Moqtaderi, Zarmik; Geisberg, Joseph V; Jin, Yi et al. (2013) Species-specific factors mediate extensive heterogeneity of mRNA 3' ends in yeasts. Proc Natl Acad Sci U S A 110:11073-8

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