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细菌钩帽蛋白 FlgD 负责钩组装的遗传分析。

Genetic analysis of the bacterial hook-capping protein FlgD responsible for hook assembly.

机构信息

Graduate School of Frontier Biosciences, Osaka University, 1-3 Yamadaoka, Suita, Osaka 565-0871, Japan.

PRESTO, JST, 4-1-8 Honcho, Kawaguchi, Saitama 332-0012, Japan.

出版信息

Microbiology (Reading). 2011 May;157(Pt 5):1354-1362. doi: 10.1099/mic.0.047100-0. Epub 2011 Feb 24.

Abstract

FlgD of Salmonella enterica is a 232 aa protein that acts as the hook cap to promote assembly of FlgE into the hook structure. The N-terminal 86 residues (FlgD(N)) complement flgD mutants, albeit to a small degree. However, little is known about the role of the C-terminal region of FlgD (FlgD(C)). Here we isolated pseudorevertants from Salmonella flgE mutants. About half of the extragenic mutations lay within FlgD(C) and only one in FlgD(N). These suppressor mutations prevented mutant FlgE subunits from leaking out to some degree. Two weakly motile flgD mutants encoding C-terminally truncated variants, FlgD₁₋₁₉₅ and FlgD((1-138f-s+4aa)), secreted larger amounts of FlgE into the culture medium than wild-type cells. Their hooks were shorter, and their length distributions were broader, with significant tailing towards smaller values. These results suggest that FlgD(C) contributes to efficient hook polymerization. Therefore, we propose that FlgD(N) attaches to the distal end of the hook to promote hook polymerization and that FlgD(C) blocks the exit of newly exported FlgE monomers into the culture medium, allowing FlgE to have more time to assemble into the hook.

摘要

沙门氏菌 FlgD 是一个由 232 个氨基酸组成的蛋白质,作为钩帽促进 FlgE 组装到钩状结构中。N 端的前 86 个残基(FlgD(N))可以补充 flgD 突变体,尽管程度较小。然而,FlgD 羧基端区域(FlgD(C))的作用知之甚少。在这里,我们从沙门氏菌 flgE 突变体中分离出伪回复突变体。大约一半的外显子突变位于 FlgD(C)内,只有一个位于 FlgD(N)内。这些抑制突变在某种程度上阻止了突变 FlgE 亚基泄漏。两个运动能力较弱的 flgD 突变体编码羧基端截断的变体,FlgD₁₋₁₉₅ 和 FlgD((1-138f-s+4aa)),将更多的 FlgE 分泌到培养基中,而野生型细胞则分泌较少。它们的钩子更短,长度分布更宽,尾巴向较小的值延伸。这些结果表明 FlgD(C)有助于有效钩聚合。因此,我们提出 FlgD(N)附着在钩的远端以促进钩聚合,而 FlgD(C)阻止新出口的 FlgE 单体进入培养基,从而使 FlgE 有更多的时间组装到钩中。

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