Abstract

We will take a molecular genetic approach to understand the structure and function of Escherichia coli Trp aporepressor, a small (107 residue), stable protein that binds tryptophan to form an active repressor (DNA- binding) complex. We are making mutant aporepressors with each of the 2,033 possible single amino acid changes, and analyzing their phenotypes in vivo. From this collection of mutant proteins with single amino acid changes, we should be able to define which residues of aporepressor are critical for folding and dimerization, for binding corepressor (tryptophan), and for binding DNA. In addition, the phenotypes of these single changes will provide us with a database to examine various strategies for the analysis of protein structure and function, including combinatorial cassette mutagenesis and alanine scanning. In addition, we will make multiple Trp aporepressors to examine various aspects of protein structure and function in molecular detail. These include multiple mutants to study the binding of tryptophan and other indole derivatives that act as corepressors using time-resolved fluorescence and NMR spectroscopy, to study DNA binding, and to study unusual structures (e.g., homopolymeric alpha-helices) within the context of this small prokaryotic protein. We will also synthesize covalent Trp repressor, to examine the tryptophan binding pocket by spectroscopic methods in greater detail. The small size and stability of the structurally well-characterized protein, Trp aporepressor, and the multi-faceted nature of its interactions with corepressors and DNA, make the trpR gene a very attractive choice for detailed genetic analysis. Biochemical study of mutant aporepressors will provide us with an unparalleled wealth of information about the structure and function of a single regulatory protein. Understanding the relationship between the structure and function of DNA-binding proteins is central to our understanding of the regulation of gene expression at the molecular level.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
2R01GM034150-09
Application #
3284683
Study Section
Microbial Physiology and Genetics Subcommittee 2 (MBC)
Project Start
1989-07-01
Project End
1994-11-30
Budget Start
1991-12-10
Budget End
1992-11-30
Support Year
9
Fiscal Year
1992
Total Cost
Indirect Cost

  Institution

Name
California Institute of Biological Research
Department
Type
DUNS #
City
La Jolla
State
CA
Country
United States
Zip Code
92037

  Publications

Grinberg, O Y; James, P E; Swartz, H M (1998) Are there significant gradients of pO2 in cells? Adv Exp Med Biol 454:415-23
Chapman, D; Hochstrasser, R; Millar, D et al. (1995) Engineering proteins without primary sequence tryptophan residues: mutant trp repressors with aliphatic substitutions for tryptophan side chains. Gene 163:1-11
Pfau, J; Arvidson, D N; Youderian, P et al. (1994) A site-specific endonuclease derived from a mutant Trp repressor with altered DNA-binding specificity. Biochemistry 33:11391-403
Arvidson, D N; Arvidson, C G; Lawson, C L et al. (1994) The tryptophan repressor sequence is highly conserved among the Enterobacteriaceae. Nucleic Acids Res 22:1821-9
Burz, D S; Beckett, D; Benson, N et al. (1994) Self-assembly of bacteriophage lambda cI repressor: effects of single-site mutations on the monomer-dimer equilibrium. Biochemistry 33:8399-405
Benson, N; Adams, C; Youderian, P (1994) Genetic selection for mutations that impair the co-operative binding of lambda repressor. Mol Microbiol 11:567-79
Arvidson, D N; Pfau, J; Hatt, J K et al. (1993) Tryptophan super-repressors with alanine 77 changes. J Biol Chem 268:4362-9
Shapiro, M; Arvidson, D N; Pfau, J et al. (1993) The challenge-phage assay reveals differences in the binding equilibria of mutant Escherichia coli Trp super-repressors in vivo. Nucleic Acids Res 21:5661-6
Benson, N; Adams, C; Youderian, P (1992) Mutant lambda repressors with increased operator affinities reveal new, specific protein-DNA contacts. Genetics 130:17-26
Arvidson, D N; Youderian, P; Schneider, T D et al. (1991) Automated kinetic assay of beta-galactosidase activity. Biotechniques 11:733-4, 736, 738

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