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调控感受态形成途径的新型细菌素

Regulation of the competence pathway as a novel role associated with a streptococcal bacteriocin.

机构信息

Dental Research Institute, Faculty of Dentistry, University of Toronto, 124 Edward St., Toronto, Ontario M5G 1G6, Canada.

出版信息

J Bacteriol. 2011 Dec;193(23):6552-9. doi: 10.1128/JB.05968-11. Epub 2011 Oct 7.

Abstract

The oral biofilm organism Streptococcus mutans must face numerous environmental stresses to survive in its natural habitat. Under specific stresses, S. mutans expresses the competence-stimulating peptide (CSP) pheromone known to induce autolysis and facilitate the uptake and incorporation of exogenous DNA, a process called DNA transformation. We have previously demonstrated that the CSP-induced CipB bacteriocin (mutacin V) is a major factor involved in both cellular processes. Our objective in this work was to characterize the role of CipB bacteriocin during DNA transformation. Although other bacteriocin mutants were impaired in their ability to acquire DNA under CSP-induced conditions, the ΔcipB mutant was the only mutant showing a sharp decrease in transformation efficiency. The autolysis function of CipB bacteriocin does not participate in the DNA transformation process, as factors released via lysis of a subpopulation of cells did not contribute to the development of genetic competence in the surviving population. Moreover, CipB does not seem to participate in membrane depolarization to assist passage of DNA. Microarray-based expression profiling showed that under CSP-induced conditions, CipB regulated ∼130 genes, among which are the comDE locus and comR and comX genes, encoding critical factors that influence competency development in S. mutans. We also discovered that the CipI protein conferring immunity to CipB-induced autolysis also prevented the transcriptional regulatory activity of CipB. Our data suggest that besides its role in cell lysis, the S. mutans CipB bacteriocin also functions as a peptide regulator for the transcriptional control of the competence regulon.

摘要

口腔生物膜生物链球菌必须面对许多环境压力,以在其自然栖息地生存。在特定的压力下,S. mutans 表达了一种被称为诱导自溶并促进外源性 DNA 摄取和整合的信号肽(CSP)。这个过程称为 DNA 转化。我们之前已经证明,CSP 诱导的 CipB 细菌素(mutacin V)是参与这两个细胞过程的主要因素。我们在这项工作中的目标是表征 CipB 细菌素在 DNA 转化过程中的作用。尽管其他细菌素突变体在 CSP 诱导条件下获取 DNA 的能力受损,但ΔcipB 突变体是唯一表现出转化效率急剧下降的突变体。CipB 细菌素的自溶功能不参与 DNA 转化过程,因为通过细胞裂解释放的因子不会促进存活细胞群体中遗传能力的发展。此外,CipB 似乎不参与膜去极化以帮助 DNA 传递。基于微阵列的表达谱分析显示,在 CSP 诱导条件下,CipB 调节了约 130 个基因,其中包括 comDE 基因座和 comR 和 comX 基因,它们编码影响 S. mutans 形成能力的关键因素。我们还发现,赋予 cipB 诱导自溶免疫的 cipI 蛋白也阻止了 cipB 的转录调节活性。我们的数据表明,除了在细胞裂解中的作用外,S. mutans CipB 细菌素还作为一种肽调节剂,对形成能力调控子的转录调控起作用。

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