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Recombineering: A Homologous Recombination-Based Method of Genetic Engineering

机译:重组:基于同源重组的基因工程方法

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摘要

Recombineering is an efficient method of in vivo genetic engineering applicable to chromosomal as well as episomal replicons in E. coli. This method circumvents the need for most standard in vitro cloning techniques. Recombineering allows construction of DNA molecules with precise junctions without constraints being imposed by restriction enzyme site location. Bacteriophage homologous recombination proteins catalyze these recombineering reactions using double- and single-strand linear DNA substrates, so-called targeting constructs, introduced by electroporation. Gene knockouts, deletions and point mutations are readily made, gene tags can be inserted, and regions of bacterial artificial chromosomes (BACs) or the E. coli genome can be subcloned by gene retrieval using recombineering. Most of these constructs can be made within about a week's time.
机译:重组是体内基因工程的一种有效方法,适用于大肠杆菌中的染色体以及附加型复制子。该方法避免了对大多数标准体外克隆技术的需求。重组允许构建具有精确连接的DNA分子,而不受限制酶位点位置的限制。噬菌体同源重组蛋白使用通过电穿孔引入的双链和单链线性DNA底物(所谓的靶向构建体)催化这些重组反应。基因敲除,缺失和点突变很容易实现,可以插入基因标签,细菌人工染色体(BAC)或大肠杆菌基因组区域可以通过使用重组的基因检索亚克隆。这些构造大多数都可以在大约一周的时间内完成。

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