Abstract

Mutagenesis by environmental agents is believed to be an initiating event in carcinogenesis. Many environmental chemicals are metabolically converted into mutagens. Mutagenesis in cultured cells treated with exogenously supplied preformed mutagens has been studied extensively but there is little information available on mutagenesis by mutagens produced within cells at physiologically relevant levels. The intrinsic differences between cells treated with exogenous reactive metabolites and metabolically competent cells treated with metabolic precursors include both the subcellular localization and the rate of exposure to reactive metabolites. Quantitative differences in the macromolecules which are covalently modified by the reactive metabolites cause alterations in cytotoxicity and genotoxicity. The few investigations comparing genotoxicity of reactive metabolites supplied exogenously and produced endogenously demonstrated dramatic differences. Clearly, more work using metabolically competent cells which more closely resemble the in vivo exposure condition is needed. The long term goal of the current proposal is to understand the mechanisms of mutagenesis by metabolically activated environmental agents considered prime candidates for initiation of carcinogenesis in exposed human populations. The working hypothesis that the gene specific distribution of DNA adducts is enhanced in cells metabolically producing mutagens and it is the distribution of adducts that determines the toxicological response.
The specific aims are: 1. To determine the aspects of chromatin structure contributing to preferential DNA damage in expressed genes, and 2. to investigate the role of dose rate in mutagenesis and gene specific DNA damage. The proposed studies will use CYP1Al -expressing human cells and benzo[a]pyrene metabolites as a model system. Gene specific DNA damage levels determined by quantitative PCR will be compared between genes and correlated with transcription rates determined by quantitative reverse transcription PCR. Mutagenesis will be followed by HPRT mutant induction and the effect of altering dose rates will be determined. The distribution of DNA damage within the HPRT and p53 genes will be monitored by ligation mediated - PCR (LM-PCR). Mutation spectra will be determined by sequencing RT-PCR produced mutant HPRT cDNAs and correlated with DNA damage spectra. Adducted proteins will be analyzed to determine potential contributions of protein modification to the toxicological response. These studies will provide needed information elucidating the interplay between chromatin structure in active genes and dose rate in determining gene specific DNA damage by a model carcinogen. The data obtained will provide a model on which to base investigations of other bioactivated chemical carcinogens.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Environmental Health Sciences (NIEHS)
Type
Research Project (R01)
Project #
5R01ES006460-03
Application #
2882830
Study Section
Special Emphasis Panel (ZRG4-ALTX-2 (01))
Project Start
1997-03-01
Project End
1999-08-31
Budget Start
1999-03-01
Budget End
1999-08-31
Support Year
3
Fiscal Year
1999
Total Cost
Indirect Cost

  Institution

Name
Wayne State University
Department
Genetics
Type
Schools of Medicine
DUNS #
City
Detroit
State
MI
Country
United States
Zip Code
48202

  Publications

McNeely, Samuel C; Xu, Xiaogiang; Taylor, B Frazier et al. (2006) Exit from arsenite-induced mitotic arrest is p53 dependent. Environ Health Perspect 114:1401-6
O'Brien, Travis J; Jiang, Guohui; Chun, Gina et al. (2006) Incision of trivalent chromium [Cr(III)]-induced DNA damage by Bacillus caldotenax UvrABC endonuclease. Mutat Res 610:85-92
Jiang, Guo Hui; Skorvaga, Milan; Croteau, Deborah L et al. (2006) Robust incision of Benoz[a]pyrene-7,8-dihyrodiol-9,10-epoxide-DNA adducts by a recombinant thermoresistant interspecies combination UvrABC endonuclease system. Biochemistry 45:7834-43
Porter, Paul C; Clark, Denise R; McDaniel, Lisa D et al. (2006) Telomerase-immortalized human fibroblasts retain UV-induced mutagenesis and p53-mediated DNA damage responses. DNA Repair (Amst) 5:61-70
Taylor, B Frazier; McNeely, Samuel C; Miller, Heather L et al. (2006) p53 suppression of arsenite-induced mitotic catastrophe is mediated by p21CIP1/WAF1. J Pharmacol Exp Ther 318:142-51
Porter, Paul C; Mellon, Isabel; States, J Christopher (2005) XP-A cells complemented with Arg228Gln and Val234Leu polymorphic XPA alleles repair BPDE-induced DNA damage better than cells complemented with the wild type allele. DNA Repair (Amst) 4:341-9
Jiang, Guohui; Jankowiak, Ryszard; Grubor, Nenad et al. (2004) Supercoiled DNA promotes formation of intercalated cis-N2-deoxyguanine adducts and base-stacked trans-N2-deoxyguanine adducts by (+)-7R,8S-dihydrodiol-9S,10R-epoxy-7,8,9,10-tetra- hydrobenzo[a]pyrene. Chem Res Toxicol 17:330-9
Jiang, GuoHui; Skorvaga, Milan; Van Houten, Bennett et al. (2003) Reduced sulfhydryls maintain specific incision of BPDE-DNA adducts by recombinant thermoresistant Bacillus caldotenax UvrABC endonuclease. Protein Expr Purif 31:88-98
States, J Christopher; Reiners Jr, John J; Pounds, Joel G et al. (2002) Arsenite disrupts mitosis and induces apoptosis in SV40-transformed human skin fibroblasts. Toxicol Appl Pharmacol 180:83-91
Cleaver, J E; Thompson, L H; Richardson, A S et al. (1999) A summary of mutations in the UV-sensitive disorders: xeroderma pigmentosum, Cockayne syndrome, and trichothiodystrophy. Hum Mutat 14:9-22

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