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通过过表达其蛋白亚基来绕过多糖外排锚复合体的亚细胞定位需求。

Bypassing the need for subcellular localization of a polysaccharide export-anchor complex by overexpressing its protein subunits.

机构信息

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

出版信息

Mol Microbiol. 2013 Jul;89(2):350-71. doi: 10.1111/mmi.12281. Epub 2013 Jun 17.

Abstract

Subcellular protein localization is thought to promote protein-protein interaction by increasing the effective concentration and enabling spatial co-ordination and proper segregation of proteins. We found that protein overexpression allowed the assembly of a productive polysaccharide biosynthesis-export-anchoring complex in the absence of polar localization in Caulobacter crescentus. Polar localization of the holdfast export protein, HfsD, depends on the presence of the other export proteins, HfsA and HfsB, and on the polar scaffold protein PodJ. The holdfast deficiency of hfsB and podJ mutants is suppressed by the overexpression of export proteins. Restored holdfasts are randomly positioned and colocalize with a holdfast anchor protein in these strains, indicating that functional complexes can form at non-polar sites. Therefore, overexpression of export proteins surpasses a concentration threshold necessary for holdfast synthesis. Restoration of holdfast synthesis at non-polar sites reduces surface adhesion, consistent with the need to spatially co-ordinate the holdfast synthesis machinery with the flagellum and pili. These strains lack the cell-specific segregation of the holdfast, resulting in the presence of holdfasts in motile daughter cells. Our results highlight the fact that multiple facets of subcellular localization can be coupled to improve the phenotypic outcome of a protein assembly.

摘要

亚细胞蛋白定位被认为可以通过增加有效浓度、促进蛋白质空间协调和适当分离来促进蛋白质-蛋白质相互作用。我们发现,在新月柄杆菌中,蛋白质过表达可以在没有极性定位的情况下组装出具有生物活性的多糖生物合成-输出-锚定复合物。附着蛋白 HfsD 的极性定位依赖于其他输出蛋白 HfsA 和 HfsB 的存在以及极性支架蛋白 PodJ。hfsB 和 podJ 突变体的附着缺陷被输出蛋白的过表达所抑制。在这些菌株中,恢复的附着是随机定位的,并与附着锚蛋白共定位,表明功能复合物可以在非极性位点形成。因此,输出蛋白的过表达超过了附着合成所需的浓度阈值。非极性位点附着合成的恢复降低了表面粘附力,这与需要将附着合成机制与鞭毛和菌毛在空间上协调一致的需求是一致的。这些菌株缺乏附着的细胞特异性分离,导致运动的子细胞中存在附着。我们的结果强调了这样一个事实,即亚细胞定位的多个方面可以被耦合起来,以改善蛋白质组装的表型结果。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/dac0/3740972/4ba125f08d76/nihms489581f1.jpg

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