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A Simple and Effective Method for Construction of Escherichia coli Strains Proficient for Genome Engineering

机译:一种简单有效的基因组工程大肠杆菌菌株的构建方法

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摘要

Multiplex genome engineering is a standalone recombineering tool for large-scale programming and accelerated evolution of cells. However, this advanced genome engineering technique has been limited to use in selected bacterial strains. We developed a simple and effective strain-independent method for effective genome engineering in Escherichia coli. The method involves introducing a suicide plasmid carrying the λ Red recombination system into the mutS gene. The suicide plasmid can be excised from the chromosome via selection in the absence of antibiotics, thus allowing transient inactivation of the mismatch repair system during genome engineering. In addition, we developed another suicide plasmid that enables integration of large DNA fragments into the lacZ genomic locus. These features enable this system to be applied in the exploitation of the benefits of genome engineering in synthetic biology, as well as the metabolic engineering of different strains of E. coli.
机译:多重基因组工程是用于大规模编程和加速细胞进化的独立重组工具。但是,这种先进的基因组工程技术仅限于在选定的细菌菌株中使用。我们开发了一种简单有效的菌株独立方法,用于大肠杆菌中的有效基因组工程。该方法包括将携带λRed重组系统的自杀质粒引入mutS基因。可以在不存在抗生素的情况下通过选择从染色体上切除自杀质粒,从而在基因组工程化过程中使错配修复系统瞬时失活。另外,我们开发了另一个自杀质粒,该质粒能够将大的DNA片段整合到lacZ基因组位点中。这些功能使该系统可用于利用基因组工程在合成生物学中的优势,以及不同大肠杆菌菌株的代谢工程。

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