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大肠杆菌提取物在体外对脱氧核糖核酸的修复作用

Deoxyribonucleic acid repair in vitro by extracts of Escherichia coli.

作者信息

Masker W E

出版信息

J Bacteriol. 1977 Mar;129(3):1415-23. doi: 10.1128/jb.129.3.1415-1423.1977.

Abstract

Deoxyribonucleic acid (DNA) from bacteriophage T7 has been used to monitor the capacity of gently lysed extracts of Escherichia coli to perform repair resynthesis after ultraviolet (UV) irradiation. Purified DNA damaged by up to 100 J of UV radiation per m2 was treated with an endonuclease from Micrococcus luteus that introduces single-strand breaks in irradiated DNA. This DNA was then used as a substrate to study repair resynthesis by extracts of E. coli. It was found that incubation with the extract and exogenous nucleoside triphosphates under suitable assay conditions resulted in removal of all pyrimidine dimers and restoration of the substrate DNA to its original molecular weight. Repair resynthesis, detected as nonconservative, UV-stimulated DNA synthesis, was directly proportional tothe number of pyrimidine dimers introduced by radiation. The repair mode described here appears to require DNA polymerase I since it does no occur at the restrictive temperature in polA12 mutants, which contain a thermolabile polymerase. The addition of purified DNA polymerase I to extracts made from a polA mutant restores the ability to complete repair at the restrictive temperature.

摘要

来自噬菌体T7的脱氧核糖核酸(DNA)已被用于监测经紫外线(UV)照射后,大肠杆菌轻度裂解提取物进行修复再合成的能力。每平方米受到高达100焦耳紫外线辐射损伤的纯化DNA,用来自藤黄微球菌的一种核酸内切酶处理,该酶会在受辐射的DNA中引入单链断裂。然后将这种DNA用作底物,以研究大肠杆菌提取物的修复再合成。结果发现,在合适的测定条件下,与提取物和外源核苷三磷酸一起孵育会导致所有嘧啶二聚体被去除,并且底物DNA恢复到其原始分子量。作为非保守性、紫外线刺激的DNA合成检测到的修复再合成,与辐射引入的嘧啶二聚体数量成正比。这里描述的修复模式似乎需要DNA聚合酶I,因为在含有热不稳定聚合酶的polA12突变体的限制温度下不会发生这种情况。向由polA突变体制备的提取物中添加纯化的DNA聚合酶I,可恢复在限制温度下完成修复的能力。

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