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经口给予巴豆醛后,采用改良的³²P后标记技术检测Fischer 344大鼠DNA中的1,N(2)-丙烷脱氧鸟苷加合物。

Detection of 1,N(2)-propanodeoxyguanosine adducts in DNA of Fischer 344 rats by an adapted (32)P-post-labeling technique after per os application of crotonaldehyde.

作者信息

Eder E

机构信息

Department of Chemistry, Faculty of Sciences, University of Indonesia, Jakarta, Indonesia.

出版信息

Carcinogenesis. 2000 Jun;21(6):1191-6.

Abstract

Crotonaldehyde is an important industrial chemical to which humans and animals are ubiquitously exposed. The main intake occurs via food, tobacco smoke and possibly also via beverages. Estimation of intake via the different routes is difficult since the data available on exposure are inconsistent. Crotonaldehyde is genotoxic, mutagenic and carcinogenic and forms 1,N(2)-propanodeoxyguanosine adducts as the main DNA adducts. We have developed a (32)P-post-labeling method for these adducts based on nuclease P1 enrichment and polyethyleneimine-cellulose TLC which allows reliable detection with a detection limit of 3 adducts/10(9) nucleotides, a labeling efficiency of 80-90% and a recovery of 38%. Using this method we found crotonaldehyde adducts in different organs of Fischer 344 rats after a single gavage of high doses of 300 and 200 mg/kg body wt in the range 0.3-3.2 +/- 0.4 adducts/10(8) nucleotides and after repeated gavage of low doses of 10 and 1 mg/kg body wt (five times a week for 6 weeks) 6.2 +/- 0.2 and 2.0 +/- 0.4 adducts/10(8)nucleotides, but not in untreated animals nor in calf thymus DNA not treated with crotonaldehyde. In contrast to our results, Chung and co-workers found adducts in tissue of untreated Fischer 344 rats. This discrepancy could depend on the different methods used but also on differences in exposure of the animals via food or due to animal housing, etc.

摘要

巴豆醛是一种重要的工业化学品,人类和动物普遍接触到它。主要摄入途径是通过食物、烟草烟雾,也可能通过饮料。由于现有的接触数据不一致,很难估计通过不同途径的摄入量。巴豆醛具有遗传毒性、致突变性和致癌性,会形成1,N(2)-丙烷脱氧鸟苷加合物作为主要的DNA加合物。我们基于核酸酶P1富集和聚乙烯亚胺-纤维素薄层层析开发了一种用于这些加合物的³²P后标记方法,该方法能够可靠检测,检测限为3个加合物/10⁹个核苷酸,标记效率为80 - 90%,回收率为38%。使用该方法,我们在单次高剂量灌胃300和200 mg/kg体重的Fischer 344大鼠的不同器官中发现了巴豆醛加合物,含量范围为0.3 - 3.2±0.4个加合物/10⁸个核苷酸,在低剂量10和1 mg/kg体重重复灌胃(每周五次,共6周)后,加合物含量分别为6.2±0.2和2.0±0.4个加合物/10⁸个核苷酸,但在未处理的动物以及未用巴豆醛处理的小牛胸腺DNA中未发现。与我们的结果相反,Chung及其同事在未处理的Fischer 344大鼠组织中发现了加合物。这种差异可能取决于所使用的不同方法,但也可能取决于动物通过食物的接触差异或由于动物饲养环境等因素。

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