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Multiphoton time-domain fluorescence lifetime imaging microscopy: practical application to protein–protein interactions using global analysis

机译:多光子时域荧光寿命成像显微镜:使用全局分析的蛋白质间相互作用的实际应用

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摘要

Förster resonance energy transfer (FRET) detected via fluorescence lifetime imaging microscopy (FLIM) and global analysis provide a way in which protein–protein interactions may be spatially localized and quantified within biological cells. The FRET efficiency and proportion of interacting molecules have been determined using bi-exponential fitting to time-domain FLIM data from a multiphoton time-correlated single-photon counting microscope system. The analysis has been made more robust to noise and significantly faster using global fitting, allowing higher spatial resolutions and/or lower acquisition times. Data have been simulated, as well as acquired from cell experiments, and the accuracy of a modified Levenberg–Marquardt fitting technique has been explored. Multi-image global analysis has been used to follow the epidermal growth factor-induced activation of Cdc42 in a short-image-interval time-lapse FLIM/FRET experiment. Our implementation offers practical analysis and time-resolved-image manipulation, which have been targeted towards providing fast execution, robustness to low photon counts, quantitative results and amenability to automation and batch processing.
机译:通过荧光寿命成像显微镜(FLIM)和整体分析检测到的Förster共振能量转移(FRET)提供了一种方法,可以在生物细胞内对蛋白质之间相互作用进行空间定位和量化。 FRET效率和相互作用分子的比例已使用双指数拟合法对来自多光子时间相关单光子计数显微镜系统的时域FLIM数据进行了确定。通过使用全局拟合,可以使分析对噪声的鲁棒性大大提高,并且可以实现更高的空间分辨率和/或更少的采集时间。已经对数据进行了模拟,以及从细胞实验中获得了数据,并且探索了改良的Levenberg-Marquardt拟合技术的准确性。在短图像间隔延时FLIM / FRET实验中,已使用多图像全局分析来跟踪表皮生长因子诱导的Cdc42活化。我们的实施方案提供了实用的分析和时间分辨图像处理,旨在提供快速执行,对低光子数量的鲁棒性,定量结果以及对自动化和批处理的适应性。

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