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多种DNA加工反应是Tn7转座的基础。

Multiple DNA processing reactions underlie Tn7 transposition.

作者信息

Gary P A, Biery M C, Bainton R J, Craig N L

机构信息

Howard Hughes Medical Institute, Department of Molecular Biology and Genetics, John Hopkins Universtiy School of Medicine, Baltimore, MD 21205, USA.

出版信息

J Mol Biol. 1996 Mar 29;257(2):301-16. doi: 10.1006/jmbi.1996.0164.

Abstract

The bacterial transposon Tn7 uses a cut and paste mechanism to translocate between non-homologous insertion sites. In the first step of recombination, double-strand breaks at each transposon end disconnect the element from the donor backbone; in the second step, the now exposed 3' transposon ends join to the target DNA. To dissect the chemical steps in these reactions, we have used mutant transposons altered at and near their extreme termini. We find that the initiating double-strand breaks result from a collaboration of two distinct DNA strand processing activities, one mediating cleavages at the 3' ends of Tn7, which can be blocked by changes at the transposon tips, and another mediating cleavages at the 5' ends. The joining of exposed 3'transposon ends to the target DNA can be blocked by changing the transposon tips. Our results suggest that the target joining step occurs through two usually concerted, but actually separable, reactions in which individual 3' transposon ends are joined to separate strands of the target DNA. Thus Tn7 transposition involves several distinct DNA processing reactions: strand cleavage and strand transfer reactions at the 3' ends of the transposon, and separate strand cleavage reactions at the 5' ends of the transposon.

摘要

细菌转座子Tn7采用剪切粘贴机制在非同源插入位点之间进行移位。在重组的第一步中,转座子两端的双链断裂使元件与供体主链断开连接;在第二步中,现在暴露的3'转座子末端与靶DNA连接。为了剖析这些反应中的化学步骤,我们使用了在其极端末端及其附近发生改变的突变转座子。我们发现起始双链断裂是由两种不同的DNA链加工活性共同作用产生的,一种介导Tn7 3'末端的切割,这种切割可被转座子末端的变化所阻断,另一种介导5'末端的切割。通过改变转座子末端,可阻断暴露的3'转座子末端与靶DNA的连接。我们的结果表明,靶连接步骤通过两个通常协同但实际上可分离的反应发生,其中单个3'转座子末端与靶DNA的不同链连接。因此,Tn7转座涉及几个不同的DNA加工反应:转座子3'末端的链切割和链转移反应,以及转座子5'末端的单独链切割反应。

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