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鼠伤寒沙门氏菌中连接鞭毛蛋白合成与鞭毛组装的负调控位点。

Negative regulatory loci coupling flagellin synthesis to flagellar assembly in Salmonella typhimurium.

作者信息

Gillen K L, Hughes K T

机构信息

Department of Microbiology, University of Washington, Seattle 98195.

出版信息

J Bacteriol. 1991 Apr;173(7):2301-10. doi: 10.1128/jb.173.7.2301-2310.1991.

DOI:10.1128/jb.173.7.2301-2310.1991
PMID:1848842
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC207783/
Abstract

The complex regulation of flagellin gene expression in Salmonella typhimurium was characterized in vivo by using lac transcriptional fusions to the two flagellin structural genes (fliC [H1] and fljB [H2]). Phase variation was measured as the rate of switching of flagellin gene expression. Switching frequencies varied from 1/500 per cell per generation to 1/10,000 per cell per generation depending on the particular insertion and the direction of switching. There is a 4- to 20-fold bias in favor of switching from the fljB(On) to the fljB(Off) orientation. Random Tn10dTc insertions were isolated which failed to express flagellin. While most of these insertions mapped to loci known to be required for flagellin expression, several new loci were identified. The presence of functional copies of all of the genes responsible for complete flagellar assembly, except the hook-associated proteins (flgK, flgL, and fliD gene products), were required for expression of the fliC or fljB flagellin genes. Two novel loci involved in negative regulation of fliC and fljB in fla mutant backgrounds were identified. One of these loci, designated the flgR locus, mapped to the flg operon at 23 min on the Salmonella linkage map. An flgR insertion mutation resulted in relief of repression of the fliC and fljB genes in all fla mutant backgrounds except for mutants in the positive regulatory loci (flhC, flhD, and fliA genes).

摘要

通过使用与两个鞭毛蛋白结构基因(fliC [H1] 和 fljB [H2])的 lac 转录融合,在体内对鼠伤寒沙门氏菌中鞭毛蛋白基因表达的复杂调控进行了表征。相变以鞭毛蛋白基因表达的切换速率来衡量。根据特定的插入和切换方向,切换频率从每细胞每代 1/500 到每细胞每代 1/10,000 不等。从 fljB(On) 切换到 fljB(Off) 方向存在 4 到 20 倍的偏向性。分离出了未能表达鞭毛蛋白的随机 Tn10dTc 插入。虽然这些插入中的大多数映射到已知对鞭毛蛋白表达必需的位点,但也鉴定出了几个新位点。除钩相关蛋白(flgK、flgL 和 fliD 基因产物)外,负责完整鞭毛组装的所有基因的功能拷贝的存在是 fliC 或 fljB 鞭毛蛋白基因表达所必需的。鉴定出了两个在 fla 突变背景下参与 fliC 和 fljB 负调控的新位点。其中一个位点,命名为 flgR 位点,映射到沙门氏菌连锁图谱上 23 分钟处的 flg 操纵子。flgR 插入突变导致除正调控位点(flhC、flhD 和 fliA 基因)的突变体外,所有 fla 突变背景下 fliC 和 fljB 基因的抑制解除。

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