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大肠杆菌中与核苷酸切除修复缺口相关的体外紫外线诱变

In vitro UV mutagenesis associated with nucleotide excision-repair gaps in Escherichia coli.

作者信息

Cohen-Fix O, Livneh Z

机构信息

Department of Biochemistry, Weizmann Institute of Science, Rehovot, Israel.

出版信息

J Biol Chem. 1994 Feb 18;269(7):4953-8.

PMID:8106470
Abstract

Using a cell-free system for UV mutagenesis we have recently shown that extracts prepared from Escherichia coli cells promote a UV mutagenesis pathway that depends on the uvrABC repair genes independent of DNA replication (type II UV mutagenesis; Cohen-Fix, O., and Livneh, Z. (1992) Proc. Natl. Acad. Sci. U.S.A. 89, 3300-3304). Type II UV mutagenesis was defective also in extracts prepared from a uvrD strain. These deficiencies were complemented by adding purified UvrA, UvrB, UvrC, or UvrD proteins to the respective cell extracts. The Uvr proteins act at an early stage in the process, probably preparing a premutagenic single-stranded DNA gap, which subsequently serves as a substrate for the mutagenic reaction. Type II UV mutagenesis was not dependent on DNA polymerases I or on DNA polymerase II, but it was dependent on DNA polymerase III. Thus, similar to the in vivo situation, only DNA polymerase III is essential for UV mutagenesis. Antibodies against the beta subunit of DNA polymerase III holoenzyme inhibited DNA replication but not UV mutagenesis. Thus, the processivity subunit of the holoenzyme is not required for type II UV mutagenesis, in agreement with a mechanism involving filling-in of short single-stranded DNA gaps.

摘要

我们最近利用无细胞系统进行紫外线诱变实验,结果表明,从大肠杆菌细胞中制备的提取物能促进一种依赖于uvrABC修复基因且独立于DNA复制的紫外线诱变途径(II型紫外线诱变;科恩 - 菲克斯,O.,和利夫内,Z.(1992年)《美国国家科学院院刊》89卷,3300 - 3304页)。在从uvrD菌株制备的提取物中,II型紫外线诱变也存在缺陷。通过向相应的细胞提取物中添加纯化的UvrA、UvrB、UvrC或UvrD蛋白,这些缺陷得以弥补。Uvr蛋白在该过程的早期起作用,可能是准备一个诱变前的单链DNA缺口,随后该缺口作为诱变反应的底物。II型紫外线诱变不依赖于DNA聚合酶I或DNA聚合酶II,但依赖于DNA聚合酶III。因此,与体内情况类似,只有DNA聚合酶III对紫外线诱变至关重要。针对DNA聚合酶III全酶β亚基的抗体抑制DNA复制,但不抑制紫外线诱变。因此,全酶的持续性亚基对于II型紫外线诱变不是必需的,这与涉及填补短单链DNA缺口的机制一致。

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