DETECTION AND COMPARISON OF DNA ADDUCTS AFTER INVITRO AND INVIVO DIESEL EMISSION EXPOSURES

被引:24
作者
GALLAGHER, J
GEORGE, M
KOHAN, M
THOMPSON, C
SHANK, T
LEWTAS, J
机构
[1] ENVIRONM HLTH RES & TESTING INC,RES TRIANGLE PK,NC 27709
[2] NIEHS,NATL TOXICOL PROGRAM,RES TRIANGLE PK,NC 27709
关键词
D O I
10.2307/3431487
中图分类号
X [环境科学、安全科学];
学科分类号
08 ; 0830 ;
摘要
Development of methods to evaluate certain classes of polycyclic aromatic compounds (PAC) detected in complex mixtures to which humans are exposed would greatly improVe the diagnostic potential of P-32-postlabeling analysis. Identification of DNA adduct patterns or specific exposure-related marker adducts would strengthen associations between observed DNA adducts and exposures to different environmental pollutants (e.g., kerosene, cigarette smoke, coke oven, and diesel). We have compared diesel-modified DNA adduct patterns in various in vitro and in vivo rodent model systems and compared them to DNA reactive oxidative and reductive metabolites of 1-nitropyrene. The formation of nitrated polycyclic aromatic hydrocarbon (nitrated PAH) DNA adducts, derived from the metabolism of diesel extract constituents, was enhanced relative to other PAH-derived DNA adducts via xanthine oxidase-catalyzed nitroreduction. These adducts were detectable only by the butanol extraction version of the postlabeling analysis. Five major DNA adducts were detected in human lymphocytes treated in vitro with diesel extract. A major adduct detected in human lymphocytes treated in vitro with diesel extract comigrated with a major adduct detected in lymphocyte DNA treated with benzo[a]pyrene (BaP) alone. Other adducts that co-migrated with the major BaP-derived adducts were detected in skin and lung DNA isolated from rodents topically treated with (50 mg) diesel extract and the major adduct detected in calf thymus DNA treated with rat liver S9 and diesel particle extract. Postlabeling of lung DNA isolated from rodents exposed via lung inhalation for 24 months to diesel combustion emissions resulted in the formation of a major nuclease-P1-sensitive DNA adduct that did not co-migrate with the major BaP-diol epoxide adduct. Based on its sensitivity to nuclease-P1, this adduct may be an N-substituted aryl adduct. Marker adducts detected in the various test systems presented here will assist in characterizing nuclease-P1-sensitive nitrated PAH adducts in humans.
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页码:225 / 228
页数:4
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