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纳秒荧光显微镜。单细胞中fura-2的发射动力学。

Nanosecond fluorescence microscopy. Emission kinetics of fura-2 in single cells.

作者信息

Keating S M, Wensel T G

机构信息

Department of Cell Biology, Stanford University School of Medicine, California 94305.

出版信息

Biophys J. 1991 Jan;59(1):186-202. doi: 10.1016/S0006-3495(91)82210-X.

Abstract

A microscope based time-correlated single photon counting instrument has been constructed to measure fluorescence intensity and emission anisotropy decays from fluorophores in single cells on a nanosecond time scale. The sample is excited and the emission collected using epi-illumination optics with frequency-doubled pulses from the cavity-dumped output of a synchronously pumped dye laser serving as an excitation source. Collection of decays from a single cell is possible due to the presence of an iris in the emission path that can be reduced to less than the diameter of a single cell. Using the instrument the decay of 60 nM 1,6-diphenyl-1,3,5-hexatriene was measured, demonstrating that adequate data for lifetime analysis can be recorded from fewer 10(3) molecules of the fluorophore in an illuminated volume of 23 fl. In addition, the intensity and anisotropy decays of fura-2 in single adherent cells and in suspensions of fura-2 loaded cells in suspension, although the relative amplitudes and decay constants vary somewhat from cell to cell. The results indicate that a significant but variable fraction of fura-2 is bound to relatively immobile macromolecular components in these cells.

摘要

已构建了一种基于显微镜的时间相关单光子计数仪器,用于在纳秒时间尺度上测量单细胞中荧光团的荧光强度和发射各向异性衰减。使用落射照明光学装置激发样品并收集发射光,激发源是来自同步泵浦染料激光腔倒空输出的倍频脉冲。由于发射路径中存在可变光阑,其可缩小至小于单个细胞的直径,因此可以收集单个细胞的衰减数据。使用该仪器测量了60 nM 1,6 - 二苯基 - 1,3,5 - 己三烯的衰减,表明在23飞升的照明体积中,从少于10³个荧光团分子中就可以记录到足够用于寿命分析的数据。此外,还测量了单个贴壁细胞以及悬浮的fura - 2负载细胞悬液中fura - 2的强度和各向异性衰减,尽管相对幅度和衰减常数在不同细胞之间略有差异。结果表明,在这些细胞中,相当一部分但数量可变的fura - 2与相对固定的大分子成分结合。

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