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用于表征活细胞中蛋白质动力学的扫描荧光相关光谱技术

Scanning FCS for the characterization of protein dynamics in live cells.

作者信息

Petrásek Zdenek, Ries Jonas, Schwille Petra

机构信息

Biotec, TU Dresden, Dresden, Germany.

出版信息

Methods Enzymol. 2010;472:317-43. doi: 10.1016/S0076-6879(10)72005-X.

Abstract

Scanning fluorescence correlation spectroscopy (sFCS) is the generic term for a group of fluorescence correlation techniques where the measurement volume is moved across the sample in a defined way. The introduction of scanning is motivated by its ability to alleviate or remove several distinct problems often encountered in standard FCS, and thus, to extend the range of applicability of fluorescence correlation methods in biological systems. These problems include poor statistical accuracy in measurements with slowly moving molecules, photobleaching, optical distortions affecting the calibration of the measurement volume, membrane instabilities, etc. Here, we present an overview of sFCS methods, explaining their benefits, implementation details, requirements, and limitations, as well as relations to each other. Further, we give examples of different sFCS implementations as applied to cellular systems, namely large-circle sFCS to measure protein dynamics in embryo cortex and line sFCS to measure protein diffusion and interactions in unstable membranes.

摘要

扫描荧光相关光谱技术(sFCS)是一组荧光相关技术的统称,在这些技术中,测量体积以特定方式在样品上移动。引入扫描技术的动机在于它能够缓解或消除标准FCS中经常遇到的几个不同问题,从而扩展荧光相关方法在生物系统中的应用范围。这些问题包括对移动缓慢的分子进行测量时统计精度较差、光漂白、影响测量体积校准的光学畸变、膜不稳定性等。在此,我们对sFCS方法进行概述,解释它们的优点、实施细节、要求和局限性,以及它们之间的相互关系。此外,我们给出不同sFCS应用于细胞系统的实例,即用于测量胚胎皮质中蛋白质动力学的大圆sFCS和用于测量不稳定膜中蛋白质扩散及相互作用的线sFCS。

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