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基因组扩增和启动子突变扩展了肠出血性大肠杆菌群体中依赖csgD的生物膜反应范围。

Genome amplification and promoter mutation expand the range of csgD-dependent biofilm responses in an STEC population.

作者信息

Uhlich Gaylen A, Chen Chin-Yi, Cottrell Bryan J, Andreozzi Elisa, Irwin Peter L, Nguyen Ly-Huong

机构信息

Molecular Characterization of Foodborne Pathogens Research Unit, Eastern Regional Research Center, Agricultural Research Service, U.S. Department of Agriculture, 600 East Mermaid Lane, Wyndmoor, PA, USA.

出版信息

Microbiology (Reading). 2017 Apr;163(4):611-621. doi: 10.1099/mic.0.000448. Epub 2017 Apr 13.

Abstract

Expression of the major biofilm components of E. coli, curli fimbriae and cellulose, requires the CsgD transcription factor. A complex regulatory network allows environmental control of csgD transcription and biofilm formation. However, most clinical serotype O157 : H7 strains contain prophage insertions in the csgD regulator, mlrA, or mutations in other regulators that restrict csgD expression. These barriers can be circumvented by certain compensating mutations that restore higher csgD expression. One mechanism is via csgD promoter mutations that switch sigma factor utilization. Biofilm-forming variants utilizing RpoD rather than RpoS have been identified in glycerol freezer stocks of the non-biofilm-forming food-borne outbreak strain, ATCC 43894. In this study we used whole genome sequencing and RNA-seq to study genotypic and transcriptomic differences between those strains. In addition to defining the consequences of the csgD promoter switch and identifying new csgD-controlled genes, we discovered a region of genome amplification in our laboratory stock of 43894 (designated 43894OW) that contributed to the regulation of csgD-dependent properties.

摘要

大肠杆菌主要生物膜成分卷曲菌毛和纤维素的表达需要CsgD转录因子。一个复杂的调控网络可实现对csgD转录和生物膜形成的环境控制。然而,大多数临床血清型O157 : H7菌株在csgD调节因子mlrA中存在原噬菌体插入,或在其他限制csgD表达的调节因子中存在突变。这些障碍可通过某些恢复较高csgD表达的补偿性突变来规避。一种机制是通过csgD启动子突变来切换sigma因子的利用。在非生物膜形成的食源性暴发菌株ATCC 43894的甘油冷冻保藏株中,已鉴定出利用RpoD而非RpoS的生物膜形成变体。在本研究中,我们使用全基因组测序和RNA测序来研究这些菌株之间的基因型和转录组差异。除了确定csgD启动子切换的后果并鉴定新的csgD控制基因外,我们还在我们的43894实验室保藏株(命名为43894OW)中发现了一个基因组扩增区域,该区域有助于调控csgD依赖性特性。

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