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一种用于无偏 STED-FCS 分析的直截了当的 STED 背景校正拟合模型。

A straightforward STED-background corrected fitting model for unbiased STED-FCS analyses.

机构信息

Aix Marseille Univ, CNRS, Inserm, CIML, Marseille, France.

Aix Marseille Univ, CNRS, Centrale Marseille, Institut Fresnel, Marseille, France.

出版信息

Methods. 2018 May 1;140-141:212-222. doi: 10.1016/j.ymeth.2018.02.010. Epub 2018 Feb 14.

Abstract

Combining stimulated emission depletion and fluorescence correlation spectroscopy (STED-FCS) provides a powerful and sensitive tool for studying the molecular dynamics in live cells with high spatio-temporal resolution. STED-FCS gives access to molecular diffusion characteristic at the nanoscale occurring within short period of times. However due to the incomplete suppression of fluorescence in the STED process, the STED-FCS point spread function (PSF) deviates from a Gaussian shape and challenges the analysis of the auto-correlation curves obtained by FCS. Here, we model the effect of the incomplete fluorescence suppression in STED-FCS experiments and propose a new fitting model improving the accuracy of the diffusion times and average molecule numbers measurements. The implementation of a STED module with pulsed laser source on a commercial confocal/FCS microscope allowed us to apply the STED-background corrected model to fit the STED-FCS measurements. The experimental results are in good accordance with the theoretical analysis both for the number of molecules and the diffusion time which decrease accordingly with the STED power.

摘要

结合受激发射损耗和荧光相关光谱(STED-FCS)为在高时空分辨率下研究活细胞中的分子动力学提供了一种强大而灵敏的工具。STED-FCS 可以获取在短时间内发生的纳米尺度上的分子扩散特征。然而,由于 STED 过程中荧光的不完全抑制,STED-FCS 的点扩散函数(PSF)偏离高斯形状,这给通过 FCS 获得的自相关曲线的分析带来了挑战。在这里,我们对 STED-FCS 实验中不完全荧光抑制的影响进行建模,并提出了一种新的拟合模型,提高了扩散时间和平均分子数测量的准确性。在商业共聚焦/FCS 显微镜上使用脉冲激光源实现 STED 模块,使我们能够将 STED-背景校正模型应用于拟合 STED-FCS 测量。实验结果与理论分析非常吻合,无论是分子数还是扩散时间都随着 STED 功率的增加而相应减小。

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