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来自α-亚类紫色细菌荚膜红细菌和大肠杆菌的SecA的比较表征揭示了膜和前体特异性的差异。

Comparative characterization of SecA from the alpha-subclass purple bacterium Rhodobacter capsulatus and Escherichia coli reveals differences in membrane and precursor specificity.

作者信息

Helde R, Wiesler B, Wachter E, Neubüser A, Hoffschulte H K, Hengelage T, Schimz K L, Stuart R A, Müller M

机构信息

Adolf Butenandt Institut für Physikalische Biochemie, Ludwig-Maximilians-Universität München, Munich, Germany.

出版信息

J Bacteriol. 1997 Jun;179(12):4003-12. doi: 10.1128/jb.179.12.4003-4012.1997.

Abstract

We have cloned the secA gene of the alpha-subclass purple bacterium Rhodobacter capsulatus, a close relative to the mitochondrial ancestor, and purified the protein after expression in Escherichia coli. R. capsulatus SecA contains 904 amino acids with 53% identity to E. coli and 54% identity to Caulobacter crescentus SecA. In contrast to the nearly equal partitioning of E. coli SecA between the cytosol and plasma membrane, R. capsulatus SecA is recovered predominantly from the membrane fraction. A SecA-deficient, cell-free synthesis-translocation system prepared from R. capsulatus is used to demonstrate translocation activity of the purified R. capsulatus SecA. This translocation activity is then compared to that of the E. coli counterpart by using various precursor proteins and inside-out membrane vesicles prepared from both bacteria. We find a preference of the R. capsulatus SecA for the homologous membrane vesicles whereas E. coli SecA is active with either type of membrane. Furthermore, the two SecA proteins clearly select between distinct precursor proteins. In addition, we show here for the first time that a bacterial c-type cytochrome utilizes the canonical, Sec-dependent export pathway.

摘要

我们克隆了α-亚类紫色细菌荚膜红细菌(Rhodobacter capsulatus)的secA基因,该细菌是线粒体祖先的近亲,并在大肠杆菌中表达后纯化了该蛋白。荚膜红细菌SecA含有904个氨基酸,与大肠杆菌SecA的同一性为53%,与新月柄杆菌(Caulobacter crescentus)SecA的同一性为54%。与大肠杆菌SecA在细胞质和质膜之间几乎平均分配不同,荚膜红细菌SecA主要从膜组分中回收。利用从荚膜红细菌制备的SecA缺陷型无细胞合成-转运系统来证明纯化的荚膜红细菌SecA的转运活性。然后,通过使用各种前体蛋白和从两种细菌制备的内翻膜囊泡,将这种转运活性与大肠杆菌对应物的转运活性进行比较。我们发现荚膜红细菌SecA更倾向于同源膜囊泡,而大肠杆菌SecA对两种类型的膜都有活性。此外,这两种SecA蛋白在不同的前体蛋白之间有明显的选择。此外,我们首次在此表明细菌c型细胞色素利用经典的、Sec依赖性输出途径。

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