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One-step, highly efficient site-directed mutagenesis by toxic protein selection

机译:通过有毒蛋白质选择进行一步式高效定点诱变

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摘要

A fast and efficient site-directed mutagenesis method has been developed, using the newly constructed plasmid pTPS19, which expresses the toxic CcdB protein originally encoded by the E. coli F plasmid. Once the target gene is cloned into pTPS19, desired mutations can be introduced with two primers. The first contains the desired mutation, and the second is designed to create a +1 frame shift in the ccdB gene to inactivate the CcdB protein. The mutants can be directly selected on LB plates containing IPTG, through which the toxic CcdB protein is induced, thereby eliminating cells carrying wild-type parental plasmids. Based on stringent selection through the toxic CcdB protein, mutagenesis efficiency of 90%-100% was reached even after one round of transformation.
机译:使用新构建的质粒pTPS19,开发了一种快速有效的定点诱变方法,该质粒表达最初由大肠杆菌F质粒编码的有毒CcdB蛋白。将靶基因克隆到pTPS19中后,可以用两种引物导入所需的突变。第一个包含所需的突变,第二个被设计为在ccdB基因中产生+1移码,以使CcdB蛋白失活。可以在含有IPTG的LB平板上直接选择突变体,通过该平板诱导毒性CcdB蛋白,从而消除携带野生型亲本质粒的细胞。基于通过毒性CcdB蛋白的严格选择,即使经过一轮转化,诱变效率仍达到90%-100%。

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