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通过³²P后标记法测定丙二醛修饰的2'-脱氧鸟苷-3'-单磷酸和DNA

Determination of malonaldehyde-modified 2'-deoxyguanosine-3'-monophosphate and DNA by 32P-postlabelling.

作者信息

Vaca C E, Vodicka P, Hemminki K

机构信息

Molecular Epidemiology Unit, NOVUM, Karolinska Institute, Huddinge, Sweden.

出版信息

Carcinogenesis. 1992 Apr;13(4):593-9. doi: 10.1093/carcin/13.4.593.

Abstract

The 32P-postlabelling assay was used to determine adducts arising upon the reaction of malonaldehyde with 2'-deoxyguanosine-3'-monophosphate. The adducts formed were isolated, structurally characterized and identified as 3-(2-deoxy-beta-D-erythro-pentafuranosyl)pyrimido[1,2-alpha] purin-10(3H)-one. The kinetics of phosphorylation by T4 polynucleotide kinase was studied using 500 fmol of the synthesized standard and found to reach its maximum after 1 h of incubation. A 60% labelling efficiency was obtained at low concentrations of substrate. The adducted substrate was detected at the sub-femtomolar level. Sensitivity of the adducts towards nuclease P1 3'-dephosphorylation was also tested. The same adduct could be detected from calf thymus DNA that had been reacted in vitro with malonaldehyde, and in DNA isolated from mice treated with [14C]malonaldehyde. DNA adducts formed in vitro were isolated after enzymatic digestion to mononucleotides followed by HPLC fractionation or nuclease P1 digestion of normal nucleotides. A combination of the two procedures proved to be the method of choice for the isolation of the malonaldehyde-DNA adducts formed in vivo prior to applying the 32P-postlabelling assay.

摘要

采用³²P后标记分析法来测定丙二醛与2'-脱氧鸟苷-3'-单磷酸反应生成的加合物。将形成的加合物分离、进行结构表征并鉴定为3-(2-脱氧-β-D-赤藓糖基)嘧啶并[1,2-α]嘌呤-10(3H)-酮。使用500飞摩尔合成标准品研究了T4多核苷酸激酶的磷酸化动力学,发现孵育1小时后达到最大值。在低底物浓度下获得了60%的标记效率。在亚飞摩尔水平检测到加合底物。还测试了加合物对核酸酶P1 3'-去磷酸化的敏感性。从体外与丙二醛反应的小牛胸腺DNA以及从用[¹⁴C]丙二醛处理的小鼠分离的DNA中都能检测到相同的加合物。体外形成的DNA加合物在酶消化成单核苷酸后,通过高效液相色谱分级分离或对正常核苷酸进行核酸酶P1消化来分离。在应用³²P后标记分析法之前,这两种方法的组合被证明是分离体内形成的丙二醛-DNA加合物的首选方法。

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