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在产生不含FliO的III型分泌装置的沙门氏菌突变菌株中组装鞭毛。

Assembling flagella in Salmonella mutant strains producing a type III export apparatus without FliO.

作者信息

Barker Clive S, Meshcheryakova Irina V, Inoue Tomoharu, Samatey Fadel A

机构信息

Trans-Membrane Trafficking Unit, Okinawa Institute of Science and Technology, Onna, Kunigami, Okinawa, Japan

Trans-Membrane Trafficking Unit, Okinawa Institute of Science and Technology, Onna, Kunigami, Okinawa, Japan.

出版信息

J Bacteriol. 2014 Dec;196(23):4001-11. doi: 10.1128/JB.02184-14. Epub 2014 Sep 8.

Abstract

The type III export apparatus of the Salmonella flagellum consists of six transmembrane proteins (FlhA, FlhB, FliO, FliP, FliQ, and FliR) and three soluble proteins (FliH, FliI, and FliJ). Deletion of the fliO gene creates a mutant strain that is poorly motile; however, suppressor mutations in the fliP gene can partially rescue motility. To further understand the mechanism of suppression of a fliO deletion mutation, we isolated new suppressor mutant strains with partially rescued motility. Whole-genome sequence analysis of these strains found a missense mutation that localized to the clpP gene [clpP(V20F)], which encodes the ClpP subunit of the ClpXP protease, and a synonymous mutation that localized to the fliA gene [fliA(+36T→C)], which encodes the flagellar sigma factor, σ(28). Combining these suppressor mutations with mutations in the fliP gene additively rescued motility and biosynthesis of the flagella in fliO deletion mutant strains. Motility was also rescued by an flgM deletion mutation or by plasmids carrying either the flhDC or fliA gene. The fliA(+36T→C) mutation increased mRNA translation of a fliA'-lacZ gene fusion, and immunoblot analysis revealed that the mutation increased levels of σ(28). Quantitative real-time reverse transcriptase PCR showed that either the clpP(V20F) or fliA(+36T→C) mutation rescued expression of class 3 flagellar and chemotaxis genes; still, the suppressor mutations in the fliP gene had a greater effect on bypassing the loss of fliO function. This suggests that the function of FliO is closely associated with regulation of FliP during assembly of the flagellum.

摘要

沙门氏菌鞭毛的III型输出装置由六种跨膜蛋白(FlhA、FlhB、FliO、FliP、FliQ和FliR)和三种可溶性蛋白(FliH、FliI和FliJ)组成。缺失fliO基因会产生运动能力较差的突变菌株;然而,fliP基因中的抑制突变可以部分恢复运动能力。为了进一步了解fliO缺失突变的抑制机制,我们分离出了运动能力部分恢复的新抑制突变菌株。对这些菌株进行全基因组序列分析,发现一个错义突变定位于clpP基因[clpP(V20F)],该基因编码ClpXP蛋白酶的ClpP亚基,还有一个同义突变定位于fliA基因[fliA(+36T→C)],该基因编码鞭毛sigma因子σ(28)。将这些抑制突变与fliP基因中的突变相结合,可累加性地恢复fliO缺失突变菌株的运动能力和鞭毛生物合成。通过flgM缺失突变或携带flhDC或fliA基因的质粒也可恢复运动能力。fliA(+36T→C)突变增加了fliA'-lacZ基因融合体的mRNA翻译,免疫印迹分析表明该突变增加了σ(28)的水平。定量实时逆转录PCR显示,clpP(V20F)或fliA(+36T→C)突变均可恢复3类鞭毛和趋化性基因的表达;不过,fliP基因中的抑制突变对绕过fliO功能丧失的影响更大。这表明FliO的功能在鞭毛组装过程中与FliP的调节密切相关。

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