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假定的杂合传感器激酶SypF通过作用于两个反应调节因子SypG和VpsR的上游来协调费氏弧菌中的生物膜形成。

The putative hybrid sensor kinase SypF coordinates biofilm formation in Vibrio fischeri by acting upstream of two response regulators, SypG and VpsR.

作者信息

Darnell Cynthia L, Hussa Elizabeth A, Visick Karen L

机构信息

Department of Microbiology and Immunology, Loyola University Chicago, Maywood, IL 60153, USA.

出版信息

J Bacteriol. 2008 Jul;190(14):4941-50. doi: 10.1128/JB.00197-08. Epub 2008 May 9.

Abstract

Colonization of the Hawaiian squid Euprymna scolopes by the marine bacterium Vibrio fischeri requires the symbiosis polysaccharide (syp) gene cluster, which contributes to symbiotic initiation by promoting biofilm formation on the surface of the symbiotic organ. We previously described roles for the syp-encoded response regulator SypG and an unlinked gene encoding the sensor kinase RscS in controlling syp transcription and inducing syp-dependent cell-cell aggregation phenotypes. Here, we report the involvement of an additional syp-encoded regulator, the putative sensor kinase SypF, in promoting biofilm formation. Through the isolation of an increased activity allele, sypF1, we determined that SypF can function to induce syp transcription as well as a variety of biofilm phenotypes, including wrinkled colony formation, adherence to glass, and pellicle formation. SypF1-mediated transcription of the syp cluster was entirely dependent on SypG. However, the biofilm phenotypes were reduced, not eliminated, in the sypG mutant. These phenotypes were also reduced in a mutant deleted for sypE, another syp-encoded response regulator. However, SypF1 still induced phenotypes in a sypG sypE double mutant, suggesting that SypF1 might activate another regulator(s). Our subsequent work revealed that the residual SypF1-induced biofilm formation depended on VpsR, a putative response regulator, and cellulose biosynthesis. These data support a model in which a network of regulators and at least two polysaccharide loci contribute to biofilm formation in V. fischeri.

摘要

海洋细菌费氏弧菌在夏威夷短尾鱿鱼体内的定殖需要共生多糖(syp)基因簇,该基因簇通过促进共生器官表面生物膜的形成来推动共生起始。我们之前描述了syp编码的响应调节因子SypG以及一个编码传感激酶RscS的非连锁基因在控制syp转录和诱导syp依赖的细胞间聚集表型方面所起的作用。在此,我们报告了另一个syp编码的调节因子,即假定的传感激酶SypF,在促进生物膜形成中的作用。通过分离一个活性增强的等位基因sypF1,我们确定SypF能够诱导syp转录以及多种生物膜表型,包括褶皱菌落形成、对玻璃的黏附以及菌膜形成。SypF1介导的syp基因簇转录完全依赖于SypG。然而,在sypG突变体中,生物膜表型有所减少,但并未消除。在缺失另一个syp编码的响应调节因子sypE的突变体中,这些表型也减少了。然而,SypF1在sypG sypE双突变体中仍能诱导表型,这表明SypF1可能激活了其他调节因子。我们随后的研究表明,SypF1诱导的残余生物膜形成依赖于假定的响应调节因子VpsR和纤维素生物合成。这些数据支持了一个模型,即调节因子网络和至少两个多糖基因座共同促进费氏弧菌生物膜的形成。

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