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Development of a fast and easy method for Escherichia coli genome editing with CRISPR/Cas9

机译:利用CRISPR / Cas9开发一种快速简便的大肠杆菌基因组编辑方法

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Background Microbial genome editing is a powerful tool to modify chromosome in way of deletion, insertion or replacement, which is one of the most important techniques in metabolic engineering research. The emergence of CRISPR/Cas9 technique inspires various genomic editing methods. Results In this research, the goal of development of a fast and easy method for Escherichia coli genome editing with high efficiency is pursued. For this purpose, we designed modular plasmid assembly strategy, compared effects of different length of homologous arms for recombination, and tested different sets of recombinases. The final technique we developed only requires one plasmid construction and one transformation of practice to edit a genomic locus with 3?days and minimal lab work. In addition, the single temperature sensitive plasmid is easy to eliminate for another round of editing. Especially, process of the modularized editing plasmid construction only takes 4?h. Conclusion In this study, we developed a fast and easy genome editing procedure based on CRISPR/Cas9 system that only required the work of one plasmid construction and one transformation, which allowed modification of a chromosome locus within 3?days and could be performed continuously for multiple loci.
机译:背景技术微生物基因组编辑是通过删除,插入或替换方式修改染色体的强大工具,这是代谢工程研究中最重要的技术之一。 CRISPR / Cas9技术的出现激发了各种基因组编辑方法。结果在本研究中,追求开发一种快速,高效的大肠杆菌基因组编辑方法的目标。为此,我们设计了模块化质粒组装策略,比较了不同长度的同源臂进行重组的效果,并测试了不同组的重组酶。我们开发的最终技术仅需一个质粒构建和一次实践改造,即可编辑基因组基因座,耗时3天,而实验室操作却最少。此外,单个温度敏感质粒易于消除,可进行另一轮编辑。特别地,模块化编辑质粒构建的过程仅需4小时。结论在这项研究中,我们基于CRISPR / Cas9系统开发了一种快速简便的基因组编辑程序,该程序仅需完成一个质粒构建和一次转化工作,即可在3天之内对染色体基因座进行修饰,并且可以连续进行。多个基因座。

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