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Two-chamber AFM: probing membrane proteins separating two aqueous compartments

机译:两室AFM:探测将两个水室分隔开的膜蛋白

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摘要

Biological membranes compartmentalize and define physical borders of cells. They are crowded with membrane proteins that fulfill diverse crucial functions. About one-third of all genes in organisms code for, and the majority of drugs target, membrane proteins. To combine structure and function analysis of membrane proteins, we designed a two-chamber atomic force microscopy (AFM) setup that allows investigation of membranes spanned over nanowells, therefore separating two aqueous chambers. We imaged nonsupported surface layers (S layers) of Corynebacterium glutamicum at sufficient resolution to delineate a 15 angstrom-wide protein pore. We probed the elastic and yield moduli of nonsupported membranes, giving access to the lateral interaction energy between proteins. We combined AFM and fluorescence microscopy to demonstrate the functionality of proteins in the setup by documenting proton pumping by Halobacterium salinarium purple membranes.
机译:生物膜分隔并定义细胞的物理边界。它们挤满了具有多种关键功能的膜蛋白。生物体中所有基因的大约三分之一编码膜蛋白,大多数药物靶向膜蛋白。为了结合膜蛋白的结构和功能分析,我们设计了一个两腔原子力显微镜(AFM)装置,可以研究跨纳孔的膜,因此将两个水腔分隔开。我们以足够的分辨率对谷氨酸棒杆菌的无支撑表面层(S层)进行成像,以描绘出15埃宽的蛋白孔。我们探究了非支撑膜的弹性模量和屈服模量,从而获得了蛋白质之间的横向相互作用能。我们结合了原子力显微镜和荧光显微镜,通过记录由盐杆菌盐质紫色膜质子泵入来证明蛋白质在功能中的功能。

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