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首页> 外文期刊>Methods: A Companion to Methods in Enzymology >Tracking unfolding and refolding reactions of single proteins using atomic force microscopy methods
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Tracking unfolding and refolding reactions of single proteins using atomic force microscopy methods

机译:使用原子力显微镜方法跟踪单个蛋白质的解折叠和重折叠反应

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摘要

During the last two decades single-molecule manipulation techniques such as atomic force microscopy (AFM) has risen to prominence through their unique capacity to provide fundamental information on the structure and function of biomolecules. Here we describe the use of single-molecule AFM to track protein unfolding and refolding pathways, enzymatic catalysis and the effects of osmolytes and chaperones on protein stability and folding. We will outline the principles of operation for two different AFM pulling techniques: length clamp and force-clamp and discuss prominent applications. We provide protocols for the construction of polyproteins which are amenable for AFM experiments, the preparation of different coverslips, choice and calibration of AFM cantilevers. We also discuss the selection criteria for AFM recordings, the calibration of AFM cantilevers, protein sample preparations and analysis of the obtained data.
机译:在过去的二十年中,诸如原子力显微镜(AFM)的单分子操纵技术因其提供有关生物分子的结构和功能的基本信息的独特能力而声名显赫。在这里,我们描述了使用单分子原子力显微镜跟踪蛋白质的展开和重折叠途径,酶催化作用以及渗透压和分子伴侣对蛋白质稳定性和折叠的影响。我们将概述两种不同的AFM牵引技术的操作原理:长度钳和力钳,并讨论突出的应用。我们提供适用于AFM实验的多蛋白构建,不同盖玻片的制备,AFM悬臂的选择和校准的规程。我们还讨论了AFM记录的选择标准,AFM悬臂梁的校准,蛋白质样品制备以及对所得数据的分析。

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