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From the Cover: Outer membrane protein G: Engineering a quiet pore for biosensing

机译:从封面开始:外膜蛋白G:设计一个安静的孔进行生物传感

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摘要

Bacterial outer membrane porins have a robust β-barrel structure and therefore show potential for use as stochastic sensors based on single-molecule detection. The monomeric porin OmpG is especially attractive compared with multisubunit proteins because appropriate modifications of the pore can be easily achieved by mutagenesis. However, the gating of OmpG causes transient current blockades in single-channel recordings that would interfere with analyte detection. To eliminate this spontaneous gating activity, we used molecular dynamics simulations to identify regions of OmpG implicated in the gating. Based on our findings, two approaches were used to enhance the stability of the open conformation by site-directed mutagenesis. First, the mobility of loop 6 was reduced by introducing a disulfide bond between the extracellular ends of strands β12 and β13. Second, the interstrand hydrogen bonding between strands β11 and β12 was optimized by deletion of residue D215. The OmpG porin with both stabilizing mutations exhibited a 95% reduction in gating activity. We used this mutant for the detection of adenosine diphosphate at the single-molecule level, after equipping the porin with a cyclodextrin molecular adapter, thereby demonstrating its potential for use in stochastic sensing applications.
机译:细菌外膜孔蛋白具有坚固的β桶结构,因此显示出基于单分子检测用作随机传感器的潜力。与多亚基蛋白质相比,单体孔蛋白OmpG特别具有吸引力,因为可以通过诱变轻松实现对孔的适当修饰。但是,OmpG的门控会在单通道记录中造成瞬态电流阻塞,这会干扰分析物的检测。为了消除这种自发的门控活动,我们使用了分子动力学模拟来识别与门控有关的OmpG区域。根据我们的发现,采用了两种方法通过定点诱变来增强开放构象的稳定性。首先,通过在链β12和​​β13的细胞外末端之间引入二硫键来降低环6的迁移率。其次,通过缺失残基D215来优化链β11和β12之间的链间氢键。具有两个稳定突变的OmpG孔蛋白的门控活性均降低了95%。在为孔蛋白配备环糊精分子适配器后,我们使用此突变体在单分子水平上检测二磷酸腺苷,从而证明了其在随机传感应用中的潜力。

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