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大肠杆菌RecE途径中限制刺激重组的异源双链特异性。

Heteroduplex strand-specificity in restriction-stimulated recombination by the RecE pathway of Escherichia coli.

作者信息

Silberstein Z, Shalit M, Cohen A

机构信息

Department of Molecular Genetics, Hebrew University-Hadassah Medical School, Jerusalem, Israel.

出版信息

Genetics. 1993 Mar;133(3):439-48. doi: 10.1093/genetics/133.3.439.

Abstract

The RecE recombination pathway is active in Escherichia coli recB recC sbcA mutants. To isolate and characterize products and intermediates of RecE-mediated, break-induced, intramolecular recombination, we infected recB recC sbcA mutants, expressing EcoRI endonuclease, with chimeric lambda phages that allow EcoRI-mediated release of cloned linear recombination substrates. Substrates with direct terminal repeats recombined to yield a circular product with one copy of the repeated sequence. Some recombinants were heteroallelic for the recombining markers. Markers distant to the break were recovered in the circular product at a higher frequency than markers close to the break. To examine the heteroduplex structures that may have yielded the heteroallelic recombinants, nonreplicative substrates were employed. Some of the nonreplicative recombination products contained heteroduplexes, with a strong bias for paired strands ending 3' at the break. This strand bias in heteroduplex formation is consistent with recombination models that postulate homologous pairing of protruding 3' single-stranded ends.

摘要

RecE重组途径在大肠杆菌recB recC sbcA突变体中具有活性。为了分离和表征RecE介导的、断裂诱导的分子内重组的产物和中间体,我们用允许EcoRI介导释放克隆线性重组底物的嵌合λ噬菌体感染表达EcoRI核酸内切酶的recB recC sbcA突变体。具有直接末端重复序列的底物发生重组,产生具有一份重复序列拷贝的环状产物。一些重组体在重组标记上是杂合等位基因的。与断裂点距离较远的标记在环状产物中的回收频率高于与断裂点距离较近的标记。为了检查可能产生杂合等位基因重组体的异源双链体结构,使用了非复制性底物。一些非复制性重组产物含有异源双链体,在断裂处强烈偏向于3'端配对的链。异源双链体形成中的这种链偏向与假设突出的3'单链末端同源配对的重组模型一致。

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本文引用的文献

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Hybridization between Escherichia coli and Shigella.大肠杆菌与志贺氏菌之间的杂交。
J Bacteriol. 1957 Oct;74(4):461-76. doi: 10.1128/jb.74.4.461-476.1957.
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Lambda replacement vectors carrying polylinker sequences.携带多克隆位点序列的λ置换载体。
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