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新月柄杆菌中合成粘性固着器所需基因的鉴定。

Identification of genes required for synthesis of the adhesive holdfast in Caulobacter crescentus.

作者信息

Smith Chris S, Hinz Aaron, Bodenmiller Diane, Larson David E, Brun Yves V

机构信息

Department of Biology, Indiana University, Bloomington, Indiana 47405, USA.

出版信息

J Bacteriol. 2003 Feb;185(4):1432-42. doi: 10.1128/JB.185.4.1432-1442.2003.

Abstract

Adhesion to both abiotic and biotic surfaces by the gram-negative prothescate bacterium Caulobacter crescentus is mediated by a polar organelle called the "holdfast," which enables the bacterium to form stable monolayer biofilms. The holdfast, a complex polysaccharide composed in part of N-acetylglucosamine, localizes to the tip of the stalk (a thin cylindrical extension of the cell wall and membranes). We report here the isolation of adhesion mutants with transposon insertions in an uncharacterized gene cluster involved in holdfast biogenesis (hfs) as well as in previously identified polar development genes (podJ and pleC), and the holdfast attachment genes (hfa). Clean deletions of three of the four genes in the hfs gene cluster (hfsDAB) resulted in a severe holdfast biogenesis phenotype. These mutants do not bind to surfaces or to a fluorescently labeled lectin, specific for N-acetylglucosamine. Transmission electron microscopy indicated that the hfsDAB mutants fail to synthesize a holdfast at the stalk tip. The predicted hfs gene products have significant sequence similarity to proteins necessary for exopolysaccharide export in gram-negative bacteria. HfsA has sequence similarity to GumC from Xanthomonas campestris, which is involved in exopolysaccharide export in the periplasm. HfsD has sequence similarity to Wza from Escherichia coli, an outer membrane protein involved in secretion of polysaccharide through the outer membrane. HfsB is a novel protein involved in holdfast biogenesis. These data suggest that the hfs genes play an important role in holdfast export.

摘要

革兰氏阴性的柄细菌新月柄杆菌对非生物和生物表面的黏附是由一种称为“固着器”的极性细胞器介导的,该细胞器使细菌能够形成稳定的单分子层生物膜。固着器是一种复杂的多糖,部分由N-乙酰葡糖胺组成,定位于柄的尖端(细胞壁和细胞膜的薄圆柱形延伸部分)。我们在此报告了黏附突变体的分离情况,这些突变体在参与固着器生物合成的一个未表征基因簇(hfs)以及先前鉴定的极性发育基因(podJ和pleC)和固着器附着基因(hfa)中存在转座子插入。hfs基因簇中四个基因中的三个(hfsDAB)的纯合缺失导致了严重的固着器生物合成表型。这些突变体不与表面或与对N-乙酰葡糖胺具有特异性的荧光标记凝集素结合。透射电子显微镜表明,hfsDAB突变体无法在柄尖合成固着器。预测的hfs基因产物与革兰氏阴性细菌胞外多糖输出所需的蛋白质具有显著的序列相似性。HfsA与野油菜黄单胞菌的GumC具有序列相似性,GumC参与周质中的胞外多糖输出。HfsD与大肠杆菌的Wza具有序列相似性,Wza是一种外膜蛋白,参与多糖通过外膜的分泌。HfsB是一种参与固着器生物合成的新蛋白。这些数据表明,hfs基因在固着器输出中起重要作用。

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本文引用的文献

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