首页> 美国卫生研究院文献>Environmental Health Perspectives >Inhalation exposure of rats and mice to 13-butadiene induces N6-adenine adducts of epoxybutene detected by 32P-postlabeling and HPLC.
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Inhalation exposure of rats and mice to 13-butadiene induces N6-adenine adducts of epoxybutene detected by 32P-postlabeling and HPLC.

机译:通过32P后标记和HPLC检测大鼠和小鼠吸入13-丁二烯会诱导环氧丁烯的N6-腺嘌呤加合物。

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摘要

In this paper we report DNA binding of butadiene monoepoxide, a first metabolite of 1,3-butadiene catalyzed by monooxygenases. We prepared alkylated purines as marker compounds for 32-P-postlabeling and electrochemical analysis and developed methods to measure the corresponding products. The traditional postlabeling assay was modified by incorporating a solid phase extraction column and high-performance liquid chromatography (HPLC) enrichment steps to the assay prior to labeling. The final analysis of adducted N6 adenines is based on two dimensional thin-layer chromatography (TLC) and an on-line HPLC/radioactivity analysis. The qualitative and quantitative results are based on positively identified marker compounds. Alkylated N7 guanines were released from DNA by neutral thermal hydrolysis, prepurified by HPLC, and analyzed by HPLC with a sensitive electrochemical detection procedure. By using these methods, we found alkylation of calf thymus DNA exposed to butadiene monoepoxide in vitro at adenine N6 and guanine N7 sites. Analysis of lung DNA samples from mice and rats exposed to butadiene through inhalation showed that adenine N6 adducts were formed in vivo in a dose responsive manner.
机译:在本文中,我们报告了丁二烯单环氧化物的DNA结合,丁二烯单环氧化物是由单加氧酶催化的1,3-丁二烯的首个代谢产物。我们制备了烷基化嘌呤作为32-P后标记和电化学分析的标志物,并开发了测量相应产物的方法。通过在标记之前将固相萃取柱和高效液相色谱(HPLC)富集步骤合并到该方法中,对传统的标记后检测方法进行了修改。对加成的N6腺嘌呤的最终分析是基于二维薄层色谱(TLC)和在线HPLC /放射性分析。定性和定量结果基于阳性鉴定的标记化合物。烷基化的N7鸟嘌呤通过中性热水解从DNA中释放出来,通过HPLC预纯化,并通过HPLC用灵敏的电化学检测程序进行分析。通过使用这些方法,我们发现了在腺嘌呤N6和鸟嘌呤N7位点暴露于丁二烯单环氧化物的小牛胸腺DNA的烷基化。对通过吸入暴露于丁二烯的小鼠和大鼠的肺部DNA样品进行的分析表明,腺嘌呤N6加合物是在体内以剂量反应方式形成的。

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