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单核细胞增生李斯特菌中的突变体构建及整合载体介导的基因互补

Mutant construction and integration vector-mediated gene complementation in Listeria monocytogenes.

作者信息

Azizoglu Reha Onur, Elhanafi Driss, Kathariou Sophia

机构信息

Department of Food, Bioprocessing and Nutrition Sciences, North Carolina State University, Raleigh, NC, USA.

出版信息

Methods Mol Biol. 2014;1157:201-11. doi: 10.1007/978-1-4939-0703-8_17.

Abstract

Genes that play role in stress response mechanisms and other phenotypes of bacteria can be identified by construction and screening of mutant libraries. In this chapter, we describe the construction and screening of mutant libraries of Listeria monocytogenes using a plasmid, pMC38, carrying a mariner-based transposon system (TC1/mariner) and constructed by Cao et al. (Appl Environ Microbiol 73:2758-2761, 2007). Following screening of the mutant library, putative mutants are identified and the transposon is localized, leading to identification of the genes that play possible roles in the phenotype of interest. To confirm the role of the gene in the relevant phenotype, transposon mutants are genetically complemented with the wild type gene using the site-specific temperature-sensitive integration vector pPL2, constructed by Lauer et al. (J Bacteriol 184:4177-4186, 2002).

摘要

通过构建和筛选突变体文库,可以鉴定出在细菌应激反应机制及其他表型中发挥作用的基因。在本章中,我们描述了利用质粒pMC38构建和筛选单核细胞增生李斯特菌突变体文库的方法,该质粒携带一个基于水手座的转座子系统(TC1/水手座),由Cao等人构建(《应用与环境微生物学》73:2758 - 2761, 2007)。筛选突变体文库后,鉴定出假定的突变体并定位转座子,从而鉴定出可能在感兴趣的表型中发挥作用的基因。为了证实该基因在相关表型中的作用,使用由Lauer等人构建的位点特异性温度敏感整合载体pPL2,用野生型基因对转座子突变体进行基因互补(《细菌学杂志》184:4177 - 4186, 2002)。

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