Abstract

Studies on factors that affect the rate of frame shift mutations in microsatellite sequences will be expanded. These factors include parameters of the microsatellite sequences themselves and mutations or altered expression of genes involved in the development of cancer. The P.I. is able to determine mutation rates and the nature of mutations in many different types of microsatellite sequences in a variety of cell types, using a plasmid vector through which these sequences are introduced into the host-cell genome. The microsatellite sequence is introduced into the vector, such that it disrupts the normal reading frame of a downstream neomycin-resistance (neo) coding sequence; clones are selected in which the reading frame of the neo gene has been restored as the result of insertions or deletions of integral numbers of repeat units in the microsatellite. A plasmid containing a (CA) 17-repeat has been introduced into human fibroblasts that express telomerase. They propose to determine whether mutation rates in these cells are comparable to those in normal diploid fibroblasts. If so, the P.I. will use these cells for many of the proposed studies. The investigators will ask whether a dominant-negative mutant mismatch-repair gene (hPMS2) results in elevation of mutation rates in the fibroblasts; these rates will be compared with those in a tumor cell line with a mutation in the same gene. They will also ask whether there are increases in mutation rates in CAK cells that have proceeded to anchorage-independence and/or outright malignancy. The P.I. proposes to continue work on the effects of the sequences of different repeat tracts on mutation rates. Besides, continuing work on the consequences of the presence of interruptions in pure-sequence tracts and on comparisons of the rates of deletion vs. insertion, they will analyze mutations of additional tetranucleotide repeats, complex microsatellites and small minisatellite sequences. They will undertake several studies designed to determine the effects of sequence context on microsatellite instability. These will include a set of experiments with a similar plasmid vector in the yeast Saccharomyces cerevisiae. Although the method that has been used for selection of frame shift mutations is sensitive and effective, the experiments each take several months to complete. In order to improve the efficiency with which the fluctuation tests can be carried, they will try using a gene fusion vector with green fluorescent protein as the reporter for mutations. With this marker, mutants can be selected by fluorescence-activated-cell sorting for many of the proposed studies.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA063264-07
Application #
6489289
Study Section
Mammalian Genetics Study Section (MGN)
Program Officer
Okano, Paul
Project Start
1995-07-13
Project End
2004-12-31
Budget Start
2002-01-01
Budget End
2002-12-31
Support Year
7
Fiscal Year
2002
Total Cost
$297,878
Indirect Cost

  Institution

Name
University of North Carolina Chapel Hill
Department
Pathology
Type
Schools of Medicine
DUNS #
078861598
City
Chapel Hill
State
NC
Country
United States
Zip Code
27599

  Publications

McDaid, J R; Loughery, J; Dunne, P et al. (2009) MLH1 mediates PARP-dependent cell death in response to the methylating agent N-methyl-N-nitrosourea. Br J Cancer 101:441-51
Boyer, Jayne C; Hawk, Joshua D; Stefanovic, Lela et al. (2008) Sequence-dependent effect of interruptions on microsatellite mutation rate in mismatch repair-deficient human cells. Mutat Res 640:89-96
Lehner, Kevin R; Stone, Megan M; Farber, Rosann A et al. (2007) Ninety-six haploid yeast strains with individual disruptions of open reading frames between YOR097C and YOR192C, constructed for the Saccharomyces genome deletion project, have an additional mutation in the mismatch repair gene MSH3. Genetics 177:1951-3
Hatch, Stephanie B; Lightfoot Jr, Harry M; Garwacki, Christopher P et al. (2005) Microsatellite instability testing in colorectal carcinoma: choice of markers affects sensitivity of detection of mismatch repair-deficient tumors. Clin Cancer Res 11:2180-7
Hawk, Joshua D; Stefanovic, Lela; Boyer, Jayne C et al. (2005) Variation in efficiency of DNA mismatch repair at different sites in the yeast genome. Proc Natl Acad Sci U S A 102:8639-43
Hatch, Stephanie B; Farber, Rosann A (2004) Mutation rates in the complex microsatellite MYCL1 and related simple repeats in cultured human cells. Mutat Res 545:117-26
Yamada, Nazumi A; Parker, Jennifer M; Farber, Rosann A (2003) Mutation frequency analysis of mononucleotide and dinucleotide repeats after oxidative stress. Environ Mol Mutagen 42:75-84
Yamada, N A; Castro, A; Farber, R A (2003) Variation in the extent of microsatellite instability in human cell lines with defects in different mismatch repair genes. Mutagenesis 18:277-82
Boyer, Jayne C; Yamada, Nazumi A; Roques, C Natalia et al. (2002) Sequence dependent instability of mononucleotide microsatellites in cultured mismatch repair proficient and deficient mammalian cells. Hum Mol Genet 11:707-13
Yamada, Nazumi A; Smith, Gwynedd A; Castro, Anay et al. (2002) Relative rates of insertion and deletion mutations in dinucleotide repeats of various lengths in mismatch repair proficient mouse and mismatch repair deficient human cells. Mutat Res 499:213-25

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