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A biphasic pulling force acts on transmembrane helices during translocon-mediated membrane integration

机译:在跨膜介导的膜整合过程中,双相拉力作用于跨膜螺旋

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摘要

Membrane proteins destined for insertion into the inner membrane of bacteria or the endoplasmic reticulum membrane in eukaryotic cells are synthesized by ribosomes bound to the bacterial SecYEG or the homologous eukaryotic Sec61 translocon. During co-translational membrane integration, transmembrane α-helical segments in the nascent chain exit the translocon through a lateral gate that opens toward the surrounding membrane, but the mechanism of lateral exit is not well understood. In particular, little is known about how a transmembrane helix behaves when entering and exiting the translocon. Using translation-arrest peptides from bacterial SecM proteins and from the mammalian Xbp1 protein as force sensors, we show that substantial force is exerted on a transmembrane helix at two distinct points during its transit through the translocon channel, providing direct insight into the dynamics of membrane integration.
机译:旨在插入真核细胞中细菌内膜或内质网膜的膜蛋白是由结合到细菌SecYEG或同源真核Sec61 translocon上的核糖体合成的。在共翻译膜整合过程中,新生链中的跨膜α螺旋片段通过向周围膜打开的侧门离开透膜,但对侧向退出的机制了解甚少。特别地,关于跨膜螺旋在进入和离开转座子时的行为了解甚少。使用细菌SecM蛋白和哺乳动物Xbp1蛋白的翻译抑制肽作为力传感器,我们显示跨膜螺旋在通过跨膜通道时的两个不同点上施加了很大的力,从而直接了解膜的动力学积分。

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