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Benzo(a)pyrene diolepoxide-DNA adducts detected by synchronous fluorescence spectrophotometry.
Author(s) -
Kirsi Vähäkangas,
Glennwood E. Trivers,
Marilyn Rowe,
Curtis C. Harris
Publication year - 1985
Publication title -
environmental health perspectives
Language(s) - Uncategorized
Resource type - Journals
SCImago Journal Rank - 2.257
H-Index - 282
eISSN - 1552-9924
pISSN - 0091-6765
DOI - 10.1289/ehp.8562101
Subject(s) - benzo(a)pyrene , chemistry , adduct , dna , carcinogen , fluorescence , pyrene , dna adduct , quenching (fluorescence) , benzopyrene , photochemistry , chromatography , analytical chemistry (journal) , microbiology and biotechnology , biochemistry , biology , organic chemistry , optics , physics
Using benzo(a)pyrene (BP) as a model carcinogen we are currently applying a fluorescence technique to detect the very low levels of carcinogen-DNA adducts in human populations due to environmental exposure. In synchronous fluorescence spectrophotometry for detection of BP-diol epoxide-DNA, excitation and emission wavelengths are scanned simultaneously with a fixed wavelength difference (delta lambda) of 34 nm. Compared to conventional fluorescence methods only one peak emerges because excitation and emission peaks have to match delta lambda to show. Because of the quenching effect of DNA, samples are hydrolyzed by acid. After this, BP-diol epoxide (BPDE)- -modified DNA gives a peak at the same wavelength and of the same fluorescence yield as BP-tetrols. When DNA from peripheral blood lymphocytes of 44 coke oven workers were analyzed, 10 had a sharp peak at 379. Among 36 coke oven workers from another factory, 4 had detectable levels of adducts. A much smaller percentage of samples was positive in a group of aluminum plant workers. We have also found BPDE-DNA adducts in DNA from pulmonary alveolar macrophages and peripheral blood lymphocytes from tobacco smokers and some of the nonsmokers.

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