REACTION-KINETICS OF DNA HISTONE CROSS-LINKING BY VINYL-ACETATE AND ACETALDEHYDE

被引:45
作者
KUYKENDALL, JR [1 ]
BOGDANFFY, MS [1 ]
机构
[1] DUPONT CO,HASKELL LAB TOXICOL & IND MED,DIV CHRON & BIOCHEM TOXICOL,POB 50,ELKTON RD,NEWARK,DE 19714
关键词
D O I
10.1093/carcin/13.11.2095
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
The formation and stability of DNA - protein crosslinks (DPXLs) formed by incubation of pUC13 plasmid DNA and calf thymus histones with 1 - 100 mM acetaldehyde was studied using a filter binding assay. DPXLs were formed at a rate of 127 DPXLs/plasmid molecule/mmol acetaldehyde in a reaction containing 1 mug of histones and 0.33 mug of DNA at 37-degrees-C for 1 h. Acetaldehyde-induced DPXLs were unstable at 37-degrees-C, with loss of up to 75% by 8 h. Crosslink formation was significantly higher at lower pH, with 3- and 2-fold higher levels at pH 5 and 6 respectively than at pH 7.5. Induction of DPXL formation by 1 - 100 mM vinyl acetate in the presence of rat liver microsomes was observed at 37-degrees-C over 3 h. DPXL accumulation followed S-phase enzymatic kinetics, with a rate of formation of 1.1 DPXLs/plasmid molecule/mmol vinyl acetate/mug microsomal protein/mug DNA. Vinyl acetate was unable to cause formation of DPXLs in the absence of microsomes. A carboxylesterase inhibitor, bis-(P-nitrophenyl) phosphate, was able to block DPXL formation by vinyl acetate and microsomes. This work supports the hypothesis that DPXL formation by vinyl acetate requires microsomal metabolism to acetaldehyde, which is the active crosslinking agent.
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页码:2095 / 2100
页数:6
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