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Single Molecule Fluorescence Microscopy on Planar Supported Bilayers

机译:平面支撑双分子层上的单分子荧光显微镜

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摘要

In the course of a single decade single molecule microscopy has changed from being a secluded domain shared merely by physicists with a strong background in optics and laser physics to a discipline that is now enjoying vivid attention by life-scientists of all venues 1. This is because single molecule imaging has the unique potential to reveal protein behavior in situ in living cells and uncover cellular organization with unprecedented resolution below the diffraction limit of visible light 2. Glass-supported planar lipid bilayers (SLBs) are a powerful tool to bring cells otherwise growing in suspension in close enough proximity to the glass slide so that they can be readily imaged in noise-reduced Total Internal Reflection illumination mode 3,4. They are very useful to study the protein dynamics in plasma membrane-associated events as diverse as cell-cell contact formation, endocytosis, exocytosis and immune recognition. Simple procedures are presented how to generate highly mobile protein-functionalized SLBs in a reproducible manner, how to determine protein mobility within and how to measure protein densities with the use of single molecule detection. It is shown how to construct a cost-efficient single molecule microscopy system with TIRF illumination capabilities and how to operate it in the experiment.
机译:在过去的十年中,单分子显微镜已从仅由具有光学和激光物理学背景的物理学家共享的一个隐秘领域转变为如今受到所有场所生命科学家的关注的学科 1 。这是因为单分子成像具有独特的潜力,可以在活细胞中原位揭示蛋白质行为,并以低于可见光 2 的衍射极限以前所未有的分辨率揭示细胞组织。玻璃支撑的平面脂质双层(SLB)是一种功能强大的工具,可以使悬浮生长的细胞以足够接近玻片的方式悬浮,从而可以在降低噪声的全内反射照明模式下轻松成像 3,4 。它们对于研究细胞膜接触形成,胞吞作用,胞吐作用和免疫识别等各种各样的质膜相关事件中的蛋白质动力学非常有用。介绍了简单的过程,该方法介绍了如何以可重现的方式生成高度可移动的蛋白功能化SLB,如何确定内部的蛋白迁移率以及如何使用单分子检测来测量蛋白密度。它显示了如何构建具有TIRF照明功能的经济高效的单分子显微镜系统,以及如何在实验中进行操作。

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