Abstract

The process of copying information contained in the DNA of an organism into RNA by RNA polymerase is a crucial step in the biological expression of this information. Consequently, this process is an important junction at which control of gene expression can be exerted. I propose to study a well-characterized system, the interaction of Escherichia coli RNA polymerase with one of the sites on DNA (promoters) at which it can initiate specific RNA synthesis: the PRM promoter of phage lambda, and the control of the process by the cI protein of the phage. I will focus on two regions of DNA, separating them. I wish to probe whether particular positions in each of the two regions are contacted independently of contacts at other positions, and search for determinants in these regions that make a particular step in the pathway to functional complex formation rate limiting. As the spacer DNA is not contacted directly by RNA polymerase, any effects of spacer sequence on promoter function must be transmitted through a particular structure the sequence specifics. By searching for spacer sequences that affect promoter function, we can learn not only about the way E. coli promoters function, but also about DNA sequences that might have altered and interesting structural properties of potential significance in modulating protein-DNA interactions. As model systems for studying the regulation of functional complex formation, I will study the activation of transcription from the PRM promoter by cI protein, and the sensitivity of this and other phage lambda promoters to supercoiling of the DNA. The sequence determinants that render a promoter sensitive to the above two conditions will be examined. In addition, I want to investigate whether there is a correlation (positive or negative) between sensitivity to the two effectors of transcription, as might be expected if control of open complex formation was exerted at the rate limiting step. These studies will be carried out using promoters with particular sequence alterations constructed in vitro, then cloned. Promoters will be characterized in vitro by measuring the rate of functional complex formation, in vivo by assaying a gene product driven by the promoter. With this work I hope to lay a solid foundation for further studies on the regulation of gene expression, in prokaryotes as well as eukaryotes.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM031808-06
Application #
3280130
Study Section
Microbial Physiology and Genetics Subcommittee 2 (MBC)
Project Start
1983-04-01
Project End
1990-02-28
Budget Start
1988-07-01
Budget End
1990-02-28
Support Year
6
Fiscal Year
1988
Total Cost
Indirect Cost

  Institution

Name
Case Western Reserve University
Department
Type
Schools of Medicine
DUNS #
077758407
City
Cleveland
State
OH
Country
United States
Zip Code
44106

  Publications

Saecker, Ruth M; Record Jr, M Thomas; Dehaseth, Pieter L (2011) Mechanism of bacterial transcription initiation: RNA polymerase - promoter binding, isomerization to initiation-competent open complexes, and initiation of RNA synthesis. J Mol Biol 412:754-71
Schroeder, Lisa A; Gries, Theodore J; Saecker, Ruth M et al. (2009) Evidence for a tyrosine-adenine stacking interaction and for a short-lived open intermediate subsequent to initial binding of Escherichia coli RNA polymerase to promoter DNA. J Mol Biol 385:339-49
Koo, Byoung-Mo; Rhodius, Virgil A; Nonaka, Gen et al. (2009) Reduced capacity of alternative sigmas to melt promoters ensures stringent promoter recognition. Genes Dev 23:2426-36
Schroeder, Lisa A; Karpen, Mary E; deHaseth, Pieter L (2008) Threonine 429 of Escherichia coli sigma 70 is a key participant in promoter DNA melting by RNA polymerase. J Mol Biol 376:153-65
Cook, Victoria M; Dehaseth, Pieter L (2007) Strand opening-deficient Escherichia coli RNA polymerase facilitates investigation of closed complexes with promoter DNA: effects of DNA sequence and temperature. J Biol Chem 282:21319-26
Schroeder, Lisa A; Choi, Ae-Jin; DeHaseth, Pieter L (2007) The -11A of promoter DNA and two conserved amino acids in the melting region of sigma70 both directly affect the rate limiting step in formation of the stable RNA polymerase-promoter complex, but they do not necessarily interact. Nucleic Acids Res 35:4141-53
Kourennaia, Olga V; Dehaseth, Pieter L (2007) Substitution of a highly conserved histidine in the Escherichia coli heat shock transcription factor, sigma32, affects promoter utilization in vitro and leads to overexpression of the biofilm-associated flu protein in vivo. J Bacteriol 189:8430-6
Schroeder, Lisa A; deHaseth, Pieter L (2005) Mechanistic differences in promoter DNA melting by Thermus aquaticus and Escherichia coli RNA polymerases. J Biol Chem 280:17422-9
Kourennaia, Olga V; Tsujikawa, Laura; Dehaseth, Pieter L (2005) Mutational analysis of Escherichia coli heat shock transcription factor sigma 32 reveals similarities with sigma 70 in recognition of the -35 promoter element and differences in promoter DNA melting and -10 recognition. J Bacteriol 187:6762-9
Sun, Li; Dove, Simon L; Panaghie, Gianina et al. (2004) An RNA polymerase mutant deficient in DNA melting facilitates study of activation mechanism: application to an artificial activator of transcription. J Mol Biol 343:1171-82

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