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Role of DNA ligase in the illegitimate recombination that generates lambdabio-transducing phages in Escherichia coli.

机译:DNA连接酶在非法重组中的作用该非法重组在大肠杆菌中产生lambdabio转导的噬菌体。

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摘要

We studied the role of DNA ligase in illegitimate recombination in Escherichia coli. A temperature-sensitive mutation in the lig gene reduced the frequency with which lambdabio-transducing phages were generated to 10-14% of that of wild type under UV irradiation. Reintroduction of the lig gene into this mutant restored the frequency of recombinant phage generation to that of wild type. Furthermore, overexpression of DNA ligase enhanced illegitimate recombination by 10-fold with or without UV irradiation. In addition, when DNA ligase was present in only limited amounts, UV-induced or spontaneous illegitimate recombination occurred exclusively at hotspot sites that have relatively long sequences of homology (9 or 13 bp). However, when DNA ligase was overexpressed, most of the illegitimate recombination took place at non-hotspot sites having only short sequences of homology (<4 bp). Thus, the level of ligase activity affects the frequency of illegitimate recombination, the length of sequence homology at the recombination sites, and the preference for recombination at hotspots, at least after UV irradiation. These observations support our hypothesis that the illegitimate recombination that generates lambdabio-transducing phages is mediated by the DNA break-and-join mechanism.
机译:我们研究了DNA连接酶在大肠杆菌中非法重组中的作用。 lig基因中的温度敏感突变将在紫外线照射下产生lambdabio的噬菌体的频率降低到野生型的10-14%。将lig基因重新引入该突变体中可将重组噬菌体的产生频率恢复为野生型。此外,在有或没有紫外线照射下,DNA连接酶的过表达将非法重组提高了10倍。另外,当DNA连接酶的含量有限时,紫外线诱导的或自发的非法重组仅在具有较长同源序列(9或13 bp)的热点位置发生。但是,当DNA连接酶过表达时,大多数非法重组发生在仅具有短同源序列(<4 bp)的非热点位点。因此,至少在紫外线照射之后,连接酶活性的水平会影响非法重组的频率,重组位点的序列同源性的长度以及热点的重组偏好。这些观察结果支持我们的假说,即产生lambdabio的噬菌体的非法重组是由DNA断裂和连接机制介导的。

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