Abstract

Our fundamental interest is a central biological problem -- how does the cell regulate transfer of information from gene to protein? We focus on RNA polymerase, the enzyme responsible for transcription. We view this enzyme as the ultimate target of a regulatory system that adjusts transcription in response to intracellular and extracellular signals by modulating the enzymatic functions of RNA polymerase. To understand this regulatory system, we first identify regions of RNA polymerase involved in a particular function by selecting, mapping and sequencing particular classes of mutants, or where appropriate by crosslinking. We then investigate how altering individual functions affects gene regulation. Because the subunit structure of RNA polymerase is highly conserved, our structure-function analysis, which is most feasible in E. coli, should have broad applicability. In the current granting period we will: 1. Further define the role of sigma in transcription initiation We will select mutations in sigma32 that block initiation in vivo in the presence of the wild type sigma32 and determine whether the mutants are defective in strand opening, phosphodiester bond formation or sigma release. In addition, we will further delineate the promoter recognition properties of sigma by determining which mutational changes in promoter DNA affect recognition by fragments of sigma70 and assessing the effects of alanine substitution mutations in sigma32 on promoter recognition. 2. Define the interactions between sigma and core RNA polymerase We will select point mutants in sigma32 and sigma70 that are defective in binding to core RNA polymerase and use them to obtain compensatory mutations in core RNA polymerase. Mutants will be characterized for their functional and regulatory effects. 3. Define functional domains in core RNA polymerase a) interaction with NusA. To define the site(s) on polymerase that bind NusA and allow us to further determine the role(s) of NusA in vivo, we will screen a group of RNA polymerase mutants defective in NusA dependent termination for those defective in binding or responding to NusA. b) substrate binding and translocation. To further characterize the regions that comprise the active site of RNA polymerase, we will identify and characterize in vitro mutants that are resistant to streptolydigin and mutants that elongate more slowly than wild-type. c) binding to DNA. We will use chemical crosslinking to identify regions of core RNA polymerase close to DNA during initiation, transition to elongation and elongation.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Allergy and Infectious Diseases (NIAID)
Type
Research Project (R01)
Project #
7R01AI019635-12
Application #
2060974
Study Section
Microbial Physiology and Genetics Subcommittee 2 (MBC)
Project Start
1983-01-01
Project End
1997-11-30
Budget Start
1993-12-01
Budget End
1994-11-30
Support Year
12
Fiscal Year
1994
Total Cost
Indirect Cost

  Institution

Name
University of California San Francisco
Department
Internal Medicine/Medicine
Type
Schools of Dentistry
DUNS #
073133571
City
San Francisco
State
CA
Country
United States
Zip Code
94143

  Publications

Dombroski, A J (1997) Recognition of the -10 promoter sequence by a partial polypeptide of sigma70 in vitro. J Biol Chem 272:3487-94
Heisler, L M; Feng, G; Jin, D J et al. (1996) Amino acid substitutions in the two largest subunits of Escherichia coli RNA polymerase that suppress a defective Rho termination factor affect different parts of the transcription complex. J Biol Chem 271:14572-83
Dombroski, A J; Johnson, B D; Lonetto, M et al. (1996) The sigma subunit of Escherichia coli RNA polymerase senses promoter spacing. Proc Natl Acad Sci U S A 93:8858-62
Karls, R K; Jin, D J; Donohue, T J (1993) Transcription properties of RNA polymerase holoenzymes isolated from the purple nonsulfur bacterium Rhodobacter sphaeroides. J Bacteriol 175:7629-38
Heisler, L M; Suzuki, H; Landick, R et al. (1993) Four contiguous amino acids define the target for streptolydigin resistance in the beta subunit of Escherichia coli RNA polymerase. J Biol Chem 268:25369-75
Dombroski, A J; Walter, W A; Gross, C A (1993) Amino-terminal amino acids modulate sigma-factor DNA-binding activity. Genes Dev 7:2446-55
Lonetto, M; Gribskov, M; Gross, C A (1992) The sigma 70 family: sequence conservation and evolutionary relationships. J Bacteriol 174:3843-9
Dombroski, A J; Walter, W A; Record Jr, M T et al. (1992) Polypeptides containing highly conserved regions of transcription initiation factor sigma 70 exhibit specificity of binding to promoter DNA. Cell 70:501-12
Jin, D J; Gross, C A (1991) RpoB8, a rifampicin-resistant termination-proficient RNA polymerase, has an increased Km for purine nucleotides during transcription elongation. J Biol Chem 266:14478-85
Hager, D A; Jin, D J; Burgess, R R (1990) Use of Mono Q high-resolution ion-exchange chromatography to obtain highly pure and active Escherichia coli RNA polymerase. Biochemistry 29:7890-4

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