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Analysis of Cellular Functions by Multipoint Fluorescence Correlation Spectroscopy

机译:多点荧光相关光谱法分析细胞功能

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摘要

The biophysical investigation of living cells is currently possible by single molecular detection methods such as fluorescence correlation spectroscopy (FCS). FCS is applied for measuring the dynamic mobility of target molecules in living cells; however, the conventional FCS systems still lack quantitative analysis for many regions of interests (ROI) in real time. To improve this situation, we have developed a novel multipoint FCS system (M-FCS) that can measure multipoint correlation functions in the cell simultaneously. To evaluate its performance, we measured correlation functions for rhodamine 6G (Rh6G) in homogeneous conditions and for green fluorescence protein (GFP) in HeLa cells. We conclude that M-FCS possesses reliable performance. As a pharmacological application, glucocorticoid receptor protein fused GFP (GR-GFP) was transfected in HeLa cells and FCS measurements were carried out in the cytoplasm and the nucleus simultaneously. The translocation of GR-GFP from the cytoplasm to the nucleus by ligand stimulation was observed with laser scanning microscopy (LSM) and M-FCS. Particularly in the nucleus, the slower diffusion of GR-GFP suggested molecular interactions after the translocation. These data imply that M-FCS can be applied for quantitative analysis of kinetic processes in living cells.
机译:目前,可以通过单分子检测方法(例如荧光相关光谱法(FCS))对活细胞进行生物物理研究。 FCS用于测量活细胞中目标分子的动态迁移率;但是,传统的FCS系统仍缺乏实时对许多感兴趣区域(ROI)进行定量分析的功能。为了改善这种情况,我们开发了一种新颖的多点FCS系统(M-FCS),可以同时测量小区中的多点相关函数。为了评估其性能,我们在均匀条件下测量了若丹明6G(Rh6G)和HeLa细胞中绿色荧光蛋白(GFP)的相关函数。我们得出结论,M-FCS具有可靠的性能。作为药理学应用,将糖皮质激素受体蛋白融合的GFP(GR-GFP)转染到HeLa细胞中,并同时在细胞质和细胞核中进行FCS测量。用激光扫描显微镜(LSM)和M-FCS观察到配体刺激GR-GFP从细胞质到细胞核的转运。特别是在细胞核中,GR-GFP的扩散较慢,提示易位后分子发生相互作用。这些数据表明,M-FCS可用于活细胞动力学过程的定量分析。

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