Abstract
The formation of DNA adducts, using the 32P-postlabelling assay, and induction of 7-ethoxyresorufin O-deethylase (EROD) were investigated in a primary culture of rainbow trout hepatocytes exposed to benzo[ a]pyrene (B[ a]P). Concentrations of 0.1 and 1 μ m-B[ a]P were shown to induce EROD whereas 10 μ m was an inhibitory concentration. DNA adducts were detected for 12 hr to 72 hr after exposure to 1 μ m-B[ a]P whereas EROD activity was increased 36 hr after treatment. The pattern of adducts was shown to be identical to that obtained after B[ a]P treatment of rainbow trout in vivo, as demonstrated by co-chromatography of the adducts. Pre-exposure of hepatocytes for 48 hr to β-naphthoflavone (βNF) and subsequent 24-hr exposure to 1 μ m-B[ a]P did not lead to increased DNA adduct formation although βNF treatment led to a 3.4-fold induction of EROD activity at the time of B[ a]P addition. This study suggests that primary culture of rainbow trout hepatocytes provides a suitable method for studying DNA adduct formation and its modulating factors in vitro.
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