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膜电位下KcsA通道新生活性的体外同步合成与功能检测

Concurrent In Vitro Synthesis and Functional Detection of Nascent Activity of the KcsA Channel under a Membrane Potential.

作者信息

Iwamoto Masayuki, Elfaramawy Maie A, Yamatake Mariko, Matsuura Tomoaki, Oiki Shigetoshi

机构信息

Department of Molecular Physiology and Biophysics , University of Fukui , Eiheiji-cho , Fukui 910-1193 , Japan.

Department of Biotechnology, Division of Advanced Science and Biotechnology, Graduate School of Engineering , Osaka University , Suita , Osaka 565-0871 , Japan.

出版信息

ACS Synth Biol. 2018 Apr 20;7(4):1004-1011. doi: 10.1021/acssynbio.7b00454. Epub 2018 Mar 28.

Abstract

Processes involved in the functional formation of prokaryotic membrane proteins have remained elusive. Here, we developed a new in vitro membrane protein expression system to detect nascent activities of the KcsA potassium channel in lipid bilayers under an applied membrane potential. The channel was synthesized using a reconstituted Escherichia coli-based in vitro transcription/translation system (IVTT) in a water-in-oil droplet lined by a membrane. The synthesized channels spontaneously incorporated into the membrane even without the translocon machinery (unassisted pathway) and formed functional channels with the correct orientation. The single-channel current of the first appearing nascent channel was captured, followed by the subsequent appearance of multiple channels. Notably, the first appearance time shortened substantially as the membrane potential was hyperpolarized. Under a steadily applied membrane potential, this system serves as a production line of membrane proteins via the unassisted pathway, mimicking the bacterial synthetic membrane.

摘要

原核生物膜蛋白功能形成所涉及的过程一直难以捉摸。在此,我们开发了一种新的体外膜蛋白表达系统,以检测在施加膜电位的情况下脂质双层中KcsA钾通道的新生活性。该通道是使用基于重组大肠杆菌的体外转录/翻译系统(IVTT)在由膜包裹的油包水液滴中合成的。即使没有转运体机制(无辅助途径),合成的通道也能自发地整合到膜中,并形成具有正确方向的功能性通道。首次出现的新生通道的单通道电流被捕获,随后出现多个通道。值得注意的是,随着膜电位超极化,首次出现时间大幅缩短。在稳定施加膜电位的情况下,该系统通过无辅助途径充当膜蛋白的生产线,模拟细菌合成膜。

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