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Genetic Method To Analyze Essential Genes of Escherichia coli

机译:大肠杆菌必需基因的遗传方法

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摘要

The genetic analysis of essential genes has been generally restricted to the use of conditional mutations, or inactivating chromosomal mutations, which require a complementing plasmid that must either be counterselected or lost to measure a phenotype. These approaches are limited because they do not permit the analysis of mutations suspected to affect a specific function of a protein, nor do they take advantage of the increasing abundance of structural and bioinformatics data for proteins. Using the dnaC gene as an example, we developed a genetic method that should permit the mutational analysis of other essential genes of Escherichia coli and related enterobacteria. The method consists of using a strain carrying a large deletion of the dnaC gene, which is complemented by a wild-type copy expressed from a plasmid that requires isopropyl-β-d-thiogalactopyranoside for maintenance. Under conditions in which this resident plasmid is lost, the method measures the function of a dnaC mutation encoded by a second plasmid. This methodology should be widely applicable to the genetic analysis of other essential genes.
机译:必需基因的遗传分析通常仅限于条件突变或灭活染色体突变的使用,这些条件突变或失活的染色体突变需要互补质粒,而该质粒必须被反选或丢失才能测量表型。这些方法之所以受到限制,是因为它们不允许分析怀疑影响蛋白质特定功能的突变,也不能利用蛋白质的结构和生物信息学数据日益丰富的优势。以dnaC基因为例,我们开发了一种遗传方法,该方法应允许对大肠杆菌和相关肠杆菌的其他必需基因进行突变分析。该方法包括使用携带dnaC基因大量缺失的菌株,该菌株由需要异丙基-β-d-硫代吡喃半乳糖苷维持的质粒表达的野生型拷贝所补充。在该常驻质粒丢失的条件下,该方法测量由第二质粒编码的dnaC突变的功能。该方法应广泛适用于其他必需基因的遗传分析。

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