The overall objective of this research project is to understand the
mechanism by which chromium(VI) compounds act as carcinogens. We plan
to test the following hypotheses: (1) that metabolic activation of
chromium(VI) results in "reactive intermediates" which give rise to
specific DNA lesions; (2) that the specific DNA lesions occur at defined
DNA sequences which are preferentially attacked because of their DNA
structure; and (3) that the specific chromium(VI)-induced DNA lesions
affect the normal template activity of DNA by altering DNA-protein
interactions. The following approaches which include both in vitro and
in vivo experimental systems will be used in attacking this problem:
(1) The chromium(V) and radical intermediates generated during the
metabolic activation of chromium(VI) by redox-active cellular components
will be determined. EPR spectroscopy will be used to detect chromium(V)
species and spin traps will be used to detect singlet oxygen and
hydroxyl and thiyl radical species formed upon reaction of chromium(VI)
be pretreated with xenobiotics which specifically affect the levels of
the various cellular redox components and change in the production of
the chromium(V) and radical species in various tissues will be
determined. (2) Chromium (VI)-induced DNA lesions, in the form of DNA
strand breaks, DNA cross-links, chromium-DNA adducts and radical-DNA
adducts, which result from the attack f "active intermediates" formed
during the metabolism of chromium(VI) will be determined in plasmid DNA
and restriction fragments in vitro and in mitochondrial and nuclear DNA
in vivo. These DNAs differ in size, conformation and associated
proteins, and therefore, may differ as targets for chromium(VI)-induced
DNA lesions. The sequence/conformation specificity of the chromium-DNA
adducts will be examined, and the chromium-DNA adducts will be isolated,
characterized and compared with synthetic chromium-nucleotide complexes.
Antibodies will be raised to chromium-DNA adducts isolated from the in
vitro reactions, and will be used to analyze DNA isolated from tissues
of rats and chick embryos treated with chromium(VI) in vivo. (3) The
effect of chromium-induced DNA lesions on protein-DNA interactions will
be examined. The ability of DNA polymerase to synthesize daughter DNA
strands in the presence of chromium-DNA adducts on the DNA template will
be determined. The ability of gene regulatory proteins to bind to their
specific DNA recognition elements after formation of chromium-DNA
adducts within these sequences will also be determined. The interaction
of lac repressor CAP and RNA polymerase with a DNA restriction fragment
containing the promoter and operator sequences of the E. coli lactose
operon, and interaction of glucocorticoid receptor and metal regulatory
proteins to a restriction fragment containing the matallothionein
promoter will be examined. These studies should elucidate critical
cellular pathways which lead to the carcinogenic activity of
chromium(VI) compounds.
National Institute of Environmental Health Sciences
CFDA Code
DUNS Number
041027822
UEI
EB8ASJBCFER9
Project Start Date
01-July-1994
Project End Date
30-June-1998
Budget Start Date
01-July-1995
Budget End Date
30-June-1996
Project Funding Information for 1995
Total Funding
$244,985
Direct Costs
$151,991
Indirect Costs
$92,994
Year
Funding IC
FY Total Cost by IC
1995
National Institute of Environmental Health Sciences
$244,985
Year
Funding IC
FY Total Cost by IC
Sub Projects
No Sub Projects information available for 5R01ES007167-13
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