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来自动物和人类源的肠炎沙门氏菌分离株中突变频率的分布以及海德堡沙门氏菌高突变株的遗传特征分析

Distribution of mutation frequencies among Salmonella enterica isolates from animal and human sources and genetic characterization of a Salmonella Heidelberg hypermutator.

作者信息

Le Gall S, Desbordes L, Gracieux P, Saffroy S, Bousarghin L, Bonnaure-Mallet M, Jolivet-Gougeon A

机构信息

Equipe Microbiologie, UPRES-EA 1254, Faculté des Sciences Pharmaceutiques et Biologiques, Université de Rennes 1, Université Européenne de Bretagne, 35043 Rennes, France.

出版信息

Vet Microbiol. 2009 Jun 12;137(3-4):306-12. doi: 10.1016/j.vetmic.2009.01.023. Epub 2009 Jan 20.

Abstract

Hypermutation is an important mechanism used by different Salmonella enterica subspecies enterica to regulate genetic stability in adaptation to changing environments, including antimicrobial treatments and industrial processes. Strong hypermutator strains generally contain a mutation in genes of the methyl mismatch repair (MMR) system and have mutation frequencies up to 1000-fold higher than wild type strains. The objectives of this study were to determine the distribution of mutation frequencies from a collection of 209 Salmonella strains, to genetically characterize a strong mutator, and to study MMR mutated protein-DNA binding interactions. Only one strain of S. Heidelberg was determined to have a hypermutator phenotype by virtue of its high mutation rate. Sequencing of genes of the MMR system showed a 12bp deletion in the mutS gene was present. The MMR mutated protein-DNA binding interactions were studied by bioanalysis, using the available crystal structure of a similar MutS protein from Escherichia coli. This analysis showed the small deletion in the Salmonella MutS was localized within the core domain. A retardation assay with MutS from hypermutable and wild type strains showed this mutation has no effect on MutS DNA binding. A better understanding of the genetic mechanisms of hypermutation will help to anticipate the behavior of hypermutator strains in various conditions.

摘要

超突变是不同肠炎沙门氏菌亚种用于调节遗传稳定性以适应不断变化的环境(包括抗菌治疗和工业过程)的重要机制。强超突变菌株通常在甲基错配修复(MMR)系统的基因中发生突变,其突变频率比野生型菌株高1000倍。本研究的目的是确定209株沙门氏菌菌株的突变频率分布,对强突变体进行遗传特征分析,并研究MMR突变蛋白与DNA的结合相互作用。通过其高突变率,仅确定一株海德堡沙门氏菌具有超突变体表型。MMR系统基因测序显示mutS基因存在12bp缺失。利用大肠杆菌中一种类似MutS蛋白的可用晶体结构,通过生物分析研究了MMR突变蛋白与DNA的结合相互作用。该分析表明,沙门氏菌MutS中的小缺失位于核心结构域内。对超突变菌株和野生型菌株的MutS进行阻滞分析表明,该突变对MutS与DNA的结合没有影响。更好地理解超突变的遗传机制将有助于预测超突变菌株在各种条件下的行为。

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