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LuxS通过一种新型调控成分控制变形链球菌中细菌素的产生。

LuxS controls bacteriocin production in Streptococcus mutans through a novel regulatory component.

作者信息

Merritt Justin, Kreth Jens, Shi Wenyuan, Qi Fengxia

机构信息

UCLA Molecular Biology Institute, Los Angeles, CA 90095, USA.

出版信息

Mol Microbiol. 2005 Aug;57(4):960-9. doi: 10.1111/j.1365-2958.2005.04733.x.

DOI:10.1111/j.1365-2958.2005.04733.x
PMID:16091037
Abstract

The oral pathogen Streptococcus mutans employs a variety of mechanisms to maintain a competitive advantage over many other oral bacteria which occupy the same ecological niche. Production of the bacteriocin, mutacin I, is one such mechanism. However, little is known about the regulatory mechanisms associated with mutacin I production. Previous work has demonstrated that the production of mutacin I greatly increased with cell density. In this study, we found that high cell density also triggered high level mutacin I gene transcription. However, this response was abolished upon deletion of luxS. Further analysis using real-time reverse transcription polymerase chain reaction (RT-PCR) demonstrated that in the luxS mutant transcription of both the mutacin I structural gene mutA and the mutacin I transcriptional activator mutR was impaired. Through microarray analysis, a putative transcription repressor annotated as Smu1274 in the Los Alamos National Laboratory Oral Pathogens Sequence Database was identified, which was strongly induced in the luxS mutant. Characterization of Smu1274, which we referred to as irvA, suggested that it may act as an inducible repressor to suppress mutacin I gene expression. A luxS and irvA double mutant regained the ability to produce mutacin I; whereas a constitutive irvA-producing strain was impaired in mutacin I production. These findings reveal a novel regulatory pathway for mutacin I gene expression, which may provide clues to the regulatory mechanisms of other cellular functions regulated by luxS in S. mutans.

摘要

口腔病原体变形链球菌采用多种机制来维持相对于占据相同生态位的许多其他口腔细菌的竞争优势。细菌素变链菌素I的产生就是这样一种机制。然而,关于与变链菌素I产生相关的调控机制知之甚少。先前的研究表明,变链菌素I的产生随着细胞密度的增加而大幅增加。在本研究中,我们发现高细胞密度也会触发变链菌素I基因的高水平转录。然而,在luxS缺失后,这种反应就消失了。使用实时逆转录聚合酶链反应(RT-PCR)进行的进一步分析表明,在luxS突变体中,变链菌素I结构基因mutA和变链菌素I转录激活因子mutR的转录均受到损害。通过微阵列分析,在洛斯阿拉莫斯国家实验室口腔病原体序列数据库中鉴定出一个假定的转录抑制因子,注释为Smu1274,它在luxS突变体中被强烈诱导。对我们称为irvA的Smu1274的表征表明,它可能作为一种诱导型抑制因子来抑制变链菌素I基因的表达。luxS和irvA双突变体恢复了产生变链菌素I的能力;而组成型产生irvA的菌株在变链菌素I产生方面受损。这些发现揭示了变链菌素I基因表达的一条新的调控途径,这可能为变形链球菌中由luxS调控的其他细胞功能的调控机制提供线索。

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