Abstract

The goals of this project are to understand how a protein binds to single-stranded nucleic acids and to understand and exploit the additivity of effects often resulting from multiple amino acid changes in a protein on its structure and function. Single-stranded nucleic acid- binding proteins play roles in key cellular processes such as DNA replication, recombination, and control of RNA translation. If the ways in which proteins interact with single-stranded nucleic acids were understood in detail, then it might be possible to modify the functions of these classes of proteins in a target fashion. This would be important in the treatment of diseases due to deficiencies in the function of these proteins. Proteins are very complex macromolecules, and engineering their properties in a completely rational manner is exceptionally difficult because the effects of changing the amino acid sequence of a protein cannot be predicted in detail. If functional and structural effects of amino acid substitutions in a protein could be accurately predicted for certain classes of multiple mutations based on the effects of the constituent single amino acid substitutions, then this process could be simplified. Such a simplification could greatly reduce the time and experimentation required to obtain a protein with a desired set of characteristics, such as a certain stability and affinity for a particular sequence of nucleic acid. The first part of this project is directed towards understanding how gene V protein interacts with single- stranded nucleic acids and how the protein preferentially recognizes a specific sequence of RNA and the cognate DNA. This is to be accomplished by determining crystal structures of complexes formed between gene V protein and oligonucleotides that bind specifically and non-specifically to the protein. We have already obtained high-quality co-crystals of two gene V protein-oligonucleotide complexes that diffract X-rays to resolutions of 3.0 angstroms and 3.4 angstroms, respectively. The goal of the second part of the project is to broaden our understanding of the additivity of effects of mutations on the structure and properties of a protein. This understanding of additivity is to be obtained by examining the effects of single and double mutations in gene V protein on the structure and properties of the protein, focusing on the relationship between the extent of additivity of effects of two mutations and the regions structurally affected by the mutations when made individually. The third part of this project is aimed at developing techniques that will allow macromolecular crystallographic experiments to be analyzed more accurately. We expect that the results of this project will have a substantial impact in the field of biotechnology and in the treatment of human disease.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM038714-13
Application #
6018702
Study Section
Special Emphasis Panel (ZRG3-BBCA (01))
Project Start
1987-07-01
Project End
2000-12-31
Budget Start
1999-08-01
Budget End
2000-12-31
Support Year
13
Fiscal Year
1999
Total Cost
Indirect Cost

  Institution

Name
Los Alamos National Lab
Department
Type
Organized Research Units
DUNS #
City
Los Alamos
State
NM
Country
United States
Zip Code
87545

  Publications

Thompson, T M; Mark, B L; Gray, C W et al. (1998) Circular dichroism and electron microscopy of a core Y61F mutant of the F1 gene 5 single-stranded DNA-binding protein and theoretical analysis of CD spectra of four Tyr --> Phe substitutions. Biochemistry 37:7463-77
Su, S; Gao, Y G; Zhang, H et al. (1997) Analyses of the stability and function of three surface mutants (R82C, K69H, and L32R) of the gene V protein from Ff phage by X-ray crystallography. Protein Sci 6:771-80
Zhang, H; Skinner, M M; Sandberg, W S et al. (1996) Context dependence of mutational effects in a protein: the crystal structures of the V35I, I47V and V35I/I47V gene V protein core mutants. J Mol Biol 259:148-59
Terwilliger, T C (1996) Gene V protein dimerization and cooperativity of binding of poly(dA). Biochemistry 35:16652-64
Mark, B L; Terwilliger, T C; Vaughan, M R et al. (1995) Circular dichroism spectroscopy of three tyrosine-to-phenylalanine substitutions of fd gene 5 protein. Biochemistry 34:12854-65
Liang, H; Sandberg, W S; Terwilliger, T C (1993) Genetic fusion of subunits of a dimeric protein substantially enhances its stability and rate of folding. Proc Natl Acad Sci U S A 90:7010-4
Liang, H; Terwilliger, T C (1991) Reversible denaturation of the gene V protein of bacteriophage f1. Biochemistry 30:2772-82
Zabin, H B; Horvath, M P; Terwilliger, T C (1991) Approaches to predicting effects of single amino acid substitutions on the function of a protein. Biochemistry 30:6230-40
Sandberg, W S; Terwilliger, T C (1989) Influence of interior packing and hydrophobicity on the stability of a protein. Science 245:54-7
Terwilliger, T C (1988) Simple and highly efficient site-specific mutagenesis, by ligation of an oligodeoxyribonucleotide into gapped heteroduplex DNA in which the template strand contains deoxyuridine. Gene 69:317-24

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