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芳香族致癌物:DNA加合物的32P后标记分析的增强灵敏度

Enhanced sensitivity of 32P-postlabeling analysis of aromatic carcinogen:DNA adducts.

作者信息

Gupta R C

出版信息

Cancer Res. 1985 Nov;45(11 Pt 2):5656-62.

PMID:4053037
Abstract

We have previously described a 32P assay for the detection and quantitation of aromatic carcinogen:DNA adducts (R. C. Gupta et al., Carcinogenesis (Lond.), 3: 1081-1092, 1982). The method entails enzymatic digestion of DNA to deoxynucleoside 3'-monophosphates which are then converted to deoxynucleoside 3',5'-[5'-32P]diphosphates by T4 polynucleotide kinase-catalyzed 32P transfer from adenosine [gamma-32P]triphosphate. Labeled adducts are purified and resolved by four-directional thin-layer chromatography. This procedure can detect one adduct in 10(7)-10(8) nucleotides but quantitation of adduct concentrations of one adduct in greater than 5 X 10(6) nucleotides becomes exceedingly difficult. I have now found that isolation of DNA adducts by extraction with 1-butanol in the presence of the phase-transfer agent tetrabutylammonium chloride prior to the labeling allows one to use excess carrier-free adenosine [gamma-32P]triphosphate (100-200 microCi), thus enabling quantitative analysis of a single adduct in 10(9)-10(10) nucleotides when 1-10 micrograms of the DNA are used. Further increase in the sensitivity of the assay requires higher amount of DNA. The four-directional thin-layer chromatography system has been modified so as to analyze simultaneously as many as 35-40 DNA samples. The new protocol, as applied to a number of carcinogenic aromatic amines and polycyclic aromatic hydrocarbons of diverse structure, is capable of detecting and quantitating adducts at the level of one adduct per 10(10) nucleotides.

摘要

我们之前描述过一种用于检测和定量芳香族致癌物

DNA加合物的32P检测法(R.C.古普塔等人,《癌变(伦敦)》,3:1081 - 1092,1982)。该方法需要将DNA酶解为脱氧核苷3'-单磷酸,然后通过T4多核苷酸激酶催化将腺苷[γ-32P]三磷酸中的32P转移,使其转化为脱氧核苷3',5'-[5'-32P]二磷酸。标记的加合物通过双向薄层层析进行纯化和分离。此程序能够检测出10(7)-10(8)个核苷酸中的一个加合物,但要对大于5×10(6)个核苷酸中的一个加合物的加合物浓度进行定量变得极其困难。我现在发现,在标记之前,在相转移剂四丁基氯化铵存在的情况下用1-丁醇萃取来分离DNA加合物,能够使用过量的无载体腺苷[γ-32P]三磷酸(100 - 200微居里),因此当使用1 - 10微克DNA时,能够对10(9)-10(10)个核苷酸中的单个加合物进行定量分析。进一步提高检测的灵敏度需要更多的DNA。双向薄层层析系统已被改进,以便能同时分析多达35 - 40个DNA样品。应用于多种结构的致癌芳香胺和多环芳烃的新方案,能够检测和定量每10(10)个核苷酸中一个加合物水平的加合物。

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