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When Coupled to Natural Transformation in Acinetobacter sp. Strain ADP1, PCR Mutagenesis Is Made Less Random by Mismatch Repair†

机译:当耦合到不动杆菌属中的自然转化时。菌株ADP1,错配修复使PCR诱变的随机性降低†

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摘要

Random PCR mutagenesis is a powerful tool for structure-function analysis of targeted proteins, especially when coupled with DNA integration through natural transformation followed by selection for loss of function. The technique has been applied successfully to structure-function analysis of transcriptional regulators, enzymes, and transporters in Acinetobacter sp. strain ADP1. However, the mismatch repair system prevents the full spectrum of nucleotide substitutions that may be selected at the level of protein function from being recovered. This barrier may be overcome by introducing PCR-mutagenized genes into strains in which the corresponding genes have been deleted.
机译:随机PCR诱变是一种功能强大的工具,可用于分析目标蛋白质的结构功能,尤其是在通过自然转化与DNA整合并随后进行功能丧失选择时,尤其如此。该技术已成功应用于不动杆菌属中转录调节因子,酶和转运蛋白的结构功能分析。菌株ADP1。但是,错配修复系统无法恢复在蛋白质功能水平上选择的核苷酸取代的全部范围。通过将PCR诱变的基因引入已删除相应基因的菌株中,可以克服这一障碍。

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