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Optimized processing and analysis of conventional confocal microscopy generated scanning FCS data

机译:传统共聚焦显微镜产生的扫描FCS数据的优化处理和分析

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摘要

Scanning Fluorescence Correlation Spectroscopy (scanning FCS) is a variant of conventional point FCS that allows molecular diffusion at multiple locations to be measured simultaneously. It enables disclosure of potential spatial heterogeneity in molecular diffusion dynamics and also the acquisition of a large amount of FCS data at the same time, providing large statistical accuracy. Here, we optimize the processing and analysis of these large-scale acquired sets of FCS data. On one hand we present FoCuS-scan, scanning FCS software that provides an end-to-end solution for processing and analysing scanning data acquired on commercial turnkey confocal systems. On the other hand, we provide a thorough characterisation of large-scale scanning FCS data over its intended time-scales and applications and propose a unique solution for the bias and variance observed when studying slowly diffusing species. Our manuscript enables researchers to straightforwardly utilise scanning FCS as a powerful technique for measuring diffusion across a broad range of physiologically relevant length scales without specialised hardware or expensive software.
机译:扫描荧光相关光谱法(扫描FCS)是常规点FCS的一种变体,它允许同时测量多个位置的分子扩散。它可以揭示分子扩散动力学中潜在的空间异质性,同时还可以获取大量的FCS数据,从而提供较大的统计准确性。在这里,我们优化了对这些大规模获取的FCS数据集的处理和分析。一方面,我们介绍了FoCuS扫描,扫描FCS软件,该软件提供了端到端解决方案,用于处理和分析在商用交钥匙共聚焦系统上获取的扫描数据。另一方面,我们提供了在预期时间范围和应用范围内大规模扫描FCS数据的全面表征,并为研究缓慢扩散物种时观察到的偏差和方差提出了独特的解决方案。我们的手稿使研究人员能够直接使用扫描FCS作为一项强大的技术,从而可以在广泛的生理相关长度范围内测量扩散,而无需专门的硬件或昂贵的软件。

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