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Single-Molecule Force Spectroscopy of Membrane Proteins from Membranes Freely Spanning Across Nanoscopic Pores

机译:跨纳米孔自由跨膜的膜蛋白的单分子力谱

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摘要

Single-molecule force spectroscopy (SMFS) provides detailed insight into the mechanical (un)folding pathways and structural stability of membrane proteins. So far, SMFS could only be applied to membrane proteins embedded in native or synthetic membranes adsorbed to solid supports. This adsorption causes experimental limitations and raises the question to what extent the support influences the results obtained by SMFS. Therefore, we introduce here SMFS from native purple membrane freely spanning across nanopores. We show that correct analysis of the SMFS data requires extending the worm-like chain model, which describes the mechanical stretching of a polypeptide, by the cubic extension model, which describes the bending of a purple membrane exposed to mechanical stress. This new experimental and theoretical approach allows to characterize the stepwise (un)folding of the membrane protein bacteriorhodopsin and to assign the stability of single and grouped secondary structures. The (un)folding and stability of bacteriorhodopsin shows no significant difference between freely spanning and directly supported purple membranes. Importantly, the novel experimental SMFS setup opens an avenue to characterize any protein from freely spanning cellular or synthetic membranes.
机译:单分子力谱(SMFS)提供了对膜蛋白的机械(解折叠)途径和结构稳定性的详细了解。到目前为止,SMFS只能应用于嵌入天然或合成膜中并吸附在固体支持物上的膜蛋白。这种吸附引起实验限制,并提出了问题,载体在多大程度上影响了SMFS获得的结果。因此,我们在这里从天然的紫色膜上自由跨过纳米孔引入SMFS。我们表明正确分析SMFS数据需要通过三次扩展模型扩展蠕虫状链模型,该模型描述多肽的机械拉伸,而三次扩展模型描述暴露于机械应力的紫色膜的弯曲。这种新的实验和理论方法可以表征膜蛋白细菌视紫红质的逐步折叠(非折叠),并确定单个和成组二级结构的稳定性。细菌视紫红质的(解折叠)和稳定性显示自由跨越的紫色膜和直接支撑的紫色膜之间没有显着差异。重要的是,新颖的实验性SMFS装置为表征自由跨越细胞膜或合成膜的任何蛋白质开辟了一条途径。

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