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羽扇豆根瘤菌H13-3和苜蓿中华根瘤菌鞭毛蛋白基因的突变分析:鞭毛蛋白A对鞭毛丝结构和转录调控的重要性

Mutational analysis of the Rhizobium lupini H13-3 and Sinorhizobium meliloti flagellin genes: importance of flagellin A for flagellar filament structure and transcriptional regulation.

作者信息

Scharf B, Schuster-Wolff-Bühring H, Rachel R, Schmitt R

机构信息

Institut für Biochemie, Genetik und Mikrobiologie, Universität Regensburg, D-93040 Regensburg, Germany.

出版信息

J Bacteriol. 2001 Sep;183(18):5334-42. doi: 10.1128/JB.183.18.5334-5342.2001.

Abstract

Complex flagellar filaments are unusual in their fine structure composed of flagellin dimers, in their right-handed helicity, and in their rigidity, which prevents a switch of handedness. The complex filaments of Rhizobium lupini H13-3 and those of Sinorhizobium meliloti are composed of three and four flagellin (Fla) subunits, respectively. The Fla-encoding genes, named flaA through flaD, are separately transcribed from sigma(28)-specific promoters. Mutational analysis of the fla genes revealed that, in both species, FlaA is the principal flagellin and that FlaB, FlaC, and FlaD are secondary. FlaA and at least one secondary Fla protein are required for assembling a functional flagellar filament. Western analysis revealed a ratio close to 1 of FlaA to the secondary Fla proteins (= FlaX) present in wild-type extracts, suggesting that the complex filament is assembled from FlaA-FlaX heterodimers. Whenever a given mutant combination of Fla prevented the assemblage of an intact filament, the biosynthesis of flagellin decreased dramatically. As shown in S. meliloti by reporter gene analysis, it is the transcription of flaA, but not of flaB, flaC, or flaD, that was down-regulated by such abortive combinations of Fla proteins. This autoregulation of flaA is unusual. We propose that any combination of Fla subunits incapable of assembling an intact filament jams the flagellar export channel and thus prevents the escape of an (as yet unidentified) anti-sigma(28) factor that antagonizes the sigma(28)-dependent transcription of flaA.

摘要

复杂鞭毛丝在其由鞭毛蛋白二聚体组成的精细结构、右手螺旋性以及阻止手性转换的刚性方面都很独特。羽扇豆根瘤菌H13-3和苜蓿中华根瘤菌的复杂鞭毛丝分别由三个和四个鞭毛蛋白(Fla)亚基组成。编码Fla的基因,命名为flaA至flaD,分别从sigma(28)特异性启动子转录。对fla基因的突变分析表明,在这两个物种中,FlaA是主要的鞭毛蛋白,而FlaB、FlaC和FlaD是次要的。组装功能性鞭毛丝需要FlaA和至少一种次要的Fla蛋白。蛋白质免疫印迹分析显示,野生型提取物中FlaA与次要Fla蛋白(=FlaX)的比例接近1,这表明复杂鞭毛丝是由FlaA-FlaX异源二聚体组装而成。每当Fla的特定突变组合阻止完整鞭毛丝的组装时,鞭毛蛋白的生物合成就会急剧下降。如在苜蓿中华根瘤菌中通过报告基因分析所示,正是flaA的转录,而不是flaB、flaC或flaD的转录,会因Fla蛋白的这种无效组合而下调。flaA的这种自动调节是不寻常的。我们提出,任何无法组装完整鞭毛丝的Fla亚基组合都会堵塞鞭毛输出通道,从而阻止一种(尚未鉴定的)抗sigma(28)因子的释放,该因子会拮抗flaA的sigma(28)依赖性转录。

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