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Measurement of nanoscale three-dimensional diffusion in the interior of living cells by STED-FCS

机译:通过STED-FCS测量活细胞内部的纳米级三维扩散

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摘要

The observation of molecular diffusion at different spatial scales, and in particular below the optical diffraction limit (<200 nm), can reveal details of the subcellular topology and its functional organization. Stimulated-emission depletion microscopy (STED) has been previously combined with fluorescence correlation spectroscopy (FCS) to investigate nanoscale diffusion (STED-FCS). However, stimulated-emission depletion fluorescence correlation spectroscopy has only been used successfully to reveal functional organization in two-dimensional space, such as the plasma membrane, while, an efficient implementation for measurements in three-dimensional space, such as the cellular interior, is still lacking. Here we integrate the STED-FCS method with two analytical approaches, the recent separation of photons by lifetime tuning and the fluorescence lifetime correlation spectroscopy, to simultaneously probe diffusion in three dimensions at different sub-diffraction scales. We demonstrate that this method efficiently provides measurement of the diffusion of EGFP at spatial scales tunable from the diffraction size down to ∼80 nm in the cytoplasm of living cells.
机译:在不同空间尺度上观察到的分子扩散,尤其是在光学衍射极限(<200 nm)以下,可以揭示亚细胞拓扑及其功能组织的细节。先前已将激发发射耗尽显微镜(STED)与荧光相关光谱(FCS)结合起来研究纳米级扩散(STED-FCS)。然而,受激发射耗尽荧光相关光谱法仅成功地用于揭示二维空间(例如质膜)中的功能组织,而在三维空间(例如细胞内部)中进行测量的有效方法是仍然缺乏。在这里,我们将STED-FCS方法与两种分析方法(最近通过寿命调整分离光子和荧光寿命相关光谱法)相结合,以同时探测不同子衍射尺度下三个维度的扩散。我们证明了这种方法有效地提供了在活细胞的细胞质中可从衍射尺寸降低至约80 nm的空间尺度上调节EGFP扩散的方法。

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