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低氯多氯联苯衍生醌形成的DNA加合物的表征与定量分析。

Characterization and quantitative analysis of DNA adducts formed from lower chlorinated PCB-derived quinones.

作者信息

Zhao Shouxun, Narang Amarjit, Ding Xinxin, Eadon George

机构信息

Department of Environmental Health and Toxicology, State University of New York at Albany, Albany, New York 12201-0509, USA.

出版信息

Chem Res Toxicol. 2004 Apr;17(4):502-11. doi: 10.1021/tx034245b.

Abstract

Polychlorinated biphenyls are wide pollutants readily detected in environmental and human specimens. DNA adduction occurs through the corresponding quinones. Polychlorinated biphenyls are first metabolized to arene oxides, which can be further oxidized to dihydroxy metabolites by microsomal cytochrome p450s. The catechol and hydroquinone products are further oxidized by peroxidases to quinones, which are electrophilic and capable of reacting with DNA to form adducts. DNA adduction is initiated by Michael addition preferentially to guanosine followed by stabilization through enolization. Another nucleophilic attack forms a five-membered ring, which aromatizes by dehydration to form the final adduct. This report describes the characterization and quantitative study of DNA adducts formed from lower chlorinated PCB-derived quinones. Quantitative study by HPLC/ESI-MS/MS and (32)P-postlabeling-HPLC gave the adduct levels in the range of 3-1200 adducts per 10(8) nucleotides. These results demonstrate that increasing chlorine substitution is associated with lower yields of DNA adduct. Although (32)P-postlabeling is more sensitive than HPLC/ESI-MS/MS for the quantitative analysis of DNA adducts, modification levels were severely underestimated by the (32)P-postlabeling assay as compared to the HPLC/ESI-MS/MS assay.

摘要

多氯联苯是广泛存在的污染物,很容易在环境和人体样本中检测到。DNA加合物通过相应的醌类形成。多氯联苯首先代谢为芳烃氧化物,后者可被微粒体细胞色素P450进一步氧化为二羟基代谢物。儿茶酚和对苯二酚产物被过氧化物酶进一步氧化为醌类,醌类具有亲电性,能够与DNA反应形成加合物。DNA加合物的形成首先是通过迈克尔加成优先作用于鸟苷,然后通过烯醇化作用实现稳定。另一次亲核攻击形成一个五元环,该五元环通过脱水芳构化形成最终的加合物。本报告描述了由低氯多氯联苯衍生的醌类形成的DNA加合物的表征和定量研究。通过HPLC/ESI-MS/MS和32P后标记-HPLC进行的定量研究得出加合物水平在每10^8个核苷酸3-1200个加合物的范围内。这些结果表明,氯取代的增加与DNA加合物的较低产率相关。尽管32P后标记法在DNA加合物的定量分析中比HPLC/ESI-MS/MS更灵敏,但与HPLC/ESI-MS/MS分析相比,32P后标记法严重低估了修饰水平。

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