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根瘤菌属基于群体感应转录调控的时间表达程序。

Temporal expression program of quorum sensing-based transcription regulation in Sinorhizobium meliloti.

机构信息

Philipps-Universität Marburg, Loewe Center for Synthetic Microbiology and Department of Biology, Marburg, Germany.

出版信息

J Bacteriol. 2013 Jul;195(14):3224-36. doi: 10.1128/JB.00234-13. Epub 2013 May 17.

Abstract

The Sin quorum sensing (QS) system of S. meliloti activates exopolysaccharide and represses flagellum production. The system consists of an N-acyl-homoserine lactone (AHL) synthase, SinI, and at least two LuxR-type regulators, SinR and ExpR. SinR appears to be independent of AHLs for its control of sinI expression, while ExpR is almost completely dependent upon AHLs. In this study, we confirmed 7 previously detected ExpR-DNA binding sites and used the consensus sequence to identify another 26 sites, some of which regulate genes previously not known to be members of the ExpR/AHL regulon. The activities of promoters dependent upon ExpR/AHL were titrated against AHL levels, with varied outcomes in AHL sensitivity. The data suggest a type of temporal expression program whereby the activity of each promoter is subject to a specific range of AHL concentrations. For example, genes responsible for exopolysaccharide production are activated at lower concentrations of AHLs than those required for the repression of genes controlling flagellum production. Several features of ExpR-regulated promoters appear to determine their response to AHLs. The location of the ExpR-binding site with respect to the relevant transcription start within each promoter region determines whether ExpR/AHL activates or represses promoter activity. Furthermore, the strength of the response is dependent upon the concentration of AHLs. We propose that this differential sensitivity to AHLs provides a bacterial colony with a transcription control program that is dynamic and precise.

摘要

根瘤菌的群体感应(QS)系统激活多糖并抑制鞭毛的产生。该系统由 N-酰基高丝氨酸内酯(AHL)合成酶 SinI 和至少两个 LuxR 型调控因子 SinR 和 ExpR 组成。SinR 似乎不依赖于 AHL 来控制 sinI 的表达,而 ExpR 几乎完全依赖于 AHL。在这项研究中,我们证实了之前检测到的 7 个 ExpR-DNA 结合位点,并使用共识序列鉴定了另外 26 个位点,其中一些调控基因以前不属于 ExpR/AHL 调控子。依赖于 ExpR/AHL 的启动子的活性与 AHL 水平相对应,AHL 敏感性的结果各不相同。数据表明存在一种时间表达程序,即每个启动子的活性受到特定范围的 AHL 浓度的影响。例如,负责多糖产生的基因在较低浓度的 AHL 下被激活,而不是那些控制鞭毛产生的基因的抑制所需要的 AHL 浓度。ExpR 调控的启动子的几个特征似乎决定了它们对 AHL 的反应。每个启动子区域内 ExpR 结合位点相对于相关转录起始的位置决定了 ExpR/AHL 是激活还是抑制启动子活性。此外,响应的强度取决于 AHL 的浓度。我们提出,这种对 AHL 的差异敏感性为细菌菌落提供了一种动态和精确的转录控制程序。

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