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Single Protein Molecule Mapping with Magnetic Atomic Force Microscopy

机译:单蛋白分子图与磁原子力显微镜

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摘要

Understanding the structural organization and distribution of proteins in biological cells is of fundamental importance in biomedical research. The use of conventional fluorescent microscopy for this purpose is limited due to its relatively low spatial resolution compared to the size of a single protein molecule. Atomic force microscopy (AFM), on the other hand, allows one to achieve single-protein resolution by scanning the cell surface using a specialized ligand-coated AFM tip. However, because this method relies on short-range interactions, it is limited to the detection of binding sites that are directly accessible to the AFM tip. We developed a method based on magnetic (long-range) interactions and applied it to investigate the structural organization and distribution of endothelin receptors on the surface of smooth muscle cells. Endothelin receptors were labeled with 50-nm superparamagnetic microbeads and then imaged with magnetic AFM. Considering its high spatial resolution and ability to “see” magnetically labeled proteins at a distance of up to 150 nm, this approach may become an important tool for investigating the dynamics of individual proteins both on the cell membrane and in the submembrane space.
机译:了解生物细胞中蛋白质的结构组织和分布在生物医学研究中至关重要。由于与单个蛋白质分子的大小相比其相对较低的空间分辨率,因此限制了常规荧光显微镜的使用。另一方面,原子力显微镜(AFM)允许通过使用专用的配体涂层AFM尖端扫描细胞表面来实现单蛋白分辨率。但是,由于此方法依赖于短程相互作用,因此仅限于检测AFM尖端可直接访问的结合位点。我们开发了一种基于磁性(远程)相互作用的方法,并将其应用于研究内皮素受体在平滑肌细胞表面的结构组织和分布。内皮素受体用50 nm超顺磁性微珠标记,然后用磁性AFM成像。考虑到它的高空间分辨率和在高达150 nm的距离上“看到”磁性标记的蛋白质的能力,这种方法可能成为研究细胞膜和膜下空间中单个蛋白质动力学的重要工具。

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