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由大肠杆菌DNA聚合酶III全酶介导的模板选择重组。

Copy-choice recombination mediated by DNA polymerase III holoenzyme from Escherichia coli.

作者信息

Canceill D, Ehrlich S D

机构信息

Laboratoire de Génétique Microbienne, Institut National de la Recherche Agronomique, Joyy-en-Josas, France.

出版信息

Proc Natl Acad Sci U S A. 1996 Jun 25;93(13):6647-52. doi: 10.1073/pnas.93.13.6647.

Abstract

Formation of deletions by recombination between short direct repeats is thought to involve either a break-join or a copy-choice process. The key step of the latter is slippage of the replication machinery between the repeats. We report that the main replicase of Escherichia coli, DNA polymerase III holoenzyme, slips between two direct repeats of 27 bp that flank an inverted repeat of approximately equal 300bp. Slippage was detected in vitro, on a single-stranded DNA template, in a primer extension assay. It requires the presence of a short (8 bp) G+C-rich sequence at the base of a hairpin that can form by annealing of the inverted repeats. It is stimulated by (i) high salt concentration, which might stabilize the hairpin, and (ii) two proteins that ensure the processivity of the DNA polymerase III holoenzyme: the single-stranded DNA binding protein and the beta subunit of the polymerase. Slippage is rather efficient under optimal reaction conditions because it can take place on >50% of template molecules. This observation supports the copy-choice model for recombination between short direct repeats.

摘要

通过短正向重复序列之间的重组形成缺失被认为涉及断裂连接或复制选择过程。后者的关键步骤是复制机制在重复序列之间的滑动。我们报告称,大肠杆菌的主要复制酶DNA聚合酶III全酶,会在两个27 bp的正向重复序列之间滑动,这两个正向重复序列位于一个约300 bp的反向重复序列两侧。在体外,在引物延伸试验中的单链DNA模板上检测到了滑动。它需要在由反向重复序列退火形成的发夹结构底部存在一个短的(8 bp)富含G + C的序列。它受到以下因素的刺激:(i)高盐浓度,这可能会稳定发夹结构;(ii)两种确保DNA聚合酶III全酶持续合成能力的蛋白质:单链DNA结合蛋白和聚合酶的β亚基。在最佳反应条件下,滑动相当高效,因为它可以在超过50%的模板分子上发生。这一观察结果支持了短正向重复序列之间重组的复制选择模型。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/81e2/39080/dc0e6e70533d/pnas01517-0445-a.jpg

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