Abstract

The molecular mechanism of gene transcription can be studied with high resolution by techniques that share a common basis in chemistry. Our overall goal for the next five years is to determine where the individual enzyme subunits bind to core RNA polymerase, DNA, and RNA in transcription complexes. Primarily this involves preparing a panel of mutants of a protein such as the E. coli alpha or sigma subunit, with each mutant containing a single reactive site for attachment of cutting reagent. This reagent, FeBABE, works by proximity, not by residue type; it selectively cleaves nearby peptide or nucleic acid backbones. Each protein conjugate will be used as a probe to cut other macromolecules in a specific complex. We shall map those residues in proteins or nucleic acids that are next to the tethered reagent at various stages of the transcription process: core enzyme, holoenzyme, binary enzyme-DNA complex, ternary enzyme-DNA-enhancer complex, ternary enzyme-DNA-RNA complex, etc. The information gained from this panel of mutants will be supplemented by other strategies, such as conjugating each with a panel of homologous cutting reagents able to cleave macromolecules over an adjustable range of distances. Taken to their logical limit, these experiments will provide a surface map of the entire complex. Developing the methodology for high resolution study of these megadalton complexes will produce tools that may find widespread use in surveying the architecture of other large molecular assemblies. These reagents are powerful probes of macromolecular structure, usable with relative ease in any system where tethered reagents are applicable. They are well suited to the study of proximity relationships in multi-subunit protein-nucleic acid complexes. The cleavage reaction is fast (seconds) , selective, and proceeds in high yield under physiological conditions. It forms products that can be characterized by standard N-terminal sequencing of the resolved peptides or by gel electrophoresis. Cleavage of proteins and nucleic acids occurs under the same conditions, permitting study of all the macromolecules involved in transcription complexes. Basic understanding of gene expression in bacteria has already formed the foundation of biotechnology; more detailed knowledge will almost certainly produce new therapeutic targets for the next generation of antibiotics.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM025909-19
Application #
6018495
Study Section
Metallobiochemistry Study Section (BMT)
Project Start
1978-12-01
Project End
2002-06-30
Budget Start
1999-07-01
Budget End
2000-06-30
Support Year
19
Fiscal Year
1999
Total Cost
Indirect Cost

  Institution

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

  Publications

Cheal, Sarah M; Ng, Mindy; Barrios, Brianda et al. (2009) Mapping protein-protein interactions by localized oxidation: consequences of the reach of hydroxyl radical. Biochemistry 48:4577-86
Lee, Susan; Young, Nicolas L; Whetstone, Paul A et al. (2006) Method to site-specifically identify and quantitate carbonyl end products of protein oxidation using oxidation-dependent element coded affinity tags (O-ECAT) and nanoliquid chromatography Fourier transform mass spectrometry. J Proteome Res 5:539-47
Whetstone, Paul A; Butlin, Nathaniel G; Corneillie, Todd M et al. (2004) Element-coded affinity tags for peptides and proteins. Bioconjug Chem 15:3-6
Schmidt, Brian D; Meares, Claude F (2002) Proteolytic DNA for mapping protein-DNA interactions. Biochemistry 41:4186-92
Marr, M T; Datwyler, S A; Meares, C F et al. (2001) Restructuring of an RNA polymerase holoenzyme elongation complex by lambdoid phage Q proteins. Proc Natl Acad Sci U S A 98:8972-8
Datwyler, S A; Meares, C F (2001) Artificial iron-dependent proteases. Met Ions Biol Syst 38:213-54
Datwyler, S A; Meares, C F (2000) Protein-protein interactions mapped by artificial proteases: where sigma factors bind to RNA polymerase. Trends Biochem Sci 25:408-14
Lee, J; Owens, J T; Hwang, I et al. (2000) Phosphorylation-induced signal propagation in the response regulator ntrC. J Bacteriol 182:5188-95
Traviglia, S L; Datwyler, S A; Yan, D et al. (1999) Targeted protein footprinting: where different transcription factors bind to RNA polymerase. Biochemistry 38:15774-8
Traviglia, S L; Datwyler, S A; Meares, C F (1999) Mapping protein-protein interactions with a library of tethered cutting reagents: the binding site of sigma 70 on Escherichia coli RNA polymerase. Biochemistry 38:4259-65

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