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Ultrastructural characterisation of Bacillus subtilis TatA complexes suggests they are too small to form homooligomeric translocation pores

机译:枯草芽孢杆菌TatA复合物的超微结构表征表明它们太小而无法形成同源寡聚易位孔

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摘要

Tat-dependent protein transport permits the traffic of fully folded proteins across membranes in bacteria and chloroplasts. The mechanism by which this occurs is not understood. Current theories propose that a key step requires the coalescence of a substrate-binding TatC-containing complex with a TatA complex, which forms pores of varying sizes that could accommodate different substrates. We have studied the structure of the TatAd complex from Bacillus subtilis using electron microscopy to generate the first 3D model of a TatA complex from a Gram-positive bacterium. We observe that TatAd does not exhibit the remarkable heterogeneity of Escherichia coli TatA complexes but instead forms ring-shaped complexes of 7.5–9 nm diameter with potential pores of 2.5–3 nm diameter that are occluded at one end. Such structures are consistent with those seen for E. coli TatE complexes. Furthermore, the small diameter of the TatAd pore, and the homogeneous nature of the complexes, suggest that TatAd cannot form the translocation channel by itself. Biochemical data indicate that another B. subtilis TatA complex, TatAc, has similar properties, suggesting a common theme for TatA-type complexes from Bacillus.
机译:依赖于Tat的蛋白质运输允许完全折叠的蛋白质跨细菌和叶绿体中的膜运输。发生这种情况的机制尚不清楚。当前的理论提出关键步骤要求将结合有底物的含TatC的复合物与TatA结合物结合,这形成了可容纳不同底物的大小不同的孔。我们使用电子显微镜研究了枯草芽孢杆菌TatAd复合物的结构,以从革兰氏阳性细菌生成TatA复合物的第一个3D模型。我们观察到,TatAd不会表现出大肠杆菌TatA复合物的显着异质性,而是会形成直径为7.5–9 nm的环状复合物,而潜在的孔径为2.5–3 nm的一端被阻塞。这种结构与大肠杆菌TatE复合物所见的结构一致。此外,TatAd孔的小直径和复合物的均质性质表明TatAd无法独自形成易位通道。生化数据表明,另一枯草芽孢杆菌TatA复合物TatAc具有相似的特性,这表明来自芽孢杆菌的TatA型复合物具有共同的主题。

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