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Time-resolved fluorescence microscopy to study biological related applications using sol-gel derived and cellular media

机译:时间分辨荧光显微镜使用溶胶-凝胶衍生和细胞培养基研究生物学相关应用

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Fluorescence microscopy provides a non-invasive means for visualising dynamic protein interactions. As well as allowing the calculation of kinetic processes via the use of time-resolved fluorescence, localisation of the protein within cells or model systems can be monitored. These fluorescence lifetime images (FLIM) have become the preferred technique for elucidating protein dynamics due to the fact that the fluorescence lifetime is an absolute measure, in the main independent of fluorophore concentration and intensity fluctuations caused by factors such as photobleaching. In this work we demonstrate the use of a time-resolved fluorescence microscopy, employing a high repetition rate laser excitation source applied to study the influence of a metal surface on fluorescence tagged protein and to elucidate viscosity using the fluorescence lifetime probe DASPMI. These were studied in a cellular environment (yeast) and in a model system based on a sol-gel derived material, in which silver nanostructures were formed in situ using irradiation from a semiconductor laser in CW mode incorporated on a compact time-resolved fluorescence microscope (HORIBA Scientific DeltaDiode and DynaMyc).
机译:荧光显微镜提供了一种非侵入性的手段来可视化动态蛋白质相互作用。除了通过使用时间分辨荧光来计算动力学过程外,还可以监测蛋白质在细胞或模型系统中的定位。这些荧光寿命图像(FLIM)已成为阐明蛋白质动力学的首选技术,这是因为荧光寿命是绝对的量度,主要独立于荧光团浓度和由诸如光漂白等因素引起的强度波动。在这项工作中,我们演示了时间分辨荧光显微镜的使用,该技术采用了高重复频率激光激发源,用于研究金属表面对荧光标记蛋白的影响并使用荧光寿命探针DASPMI阐明粘度。这些是在细胞环境(酵母)中和基于溶胶-凝胶衍生材料的模型系统中进行研究的,其中使用半导体激光器以CW模式照射并在紧凑型时间分辨荧光显微镜上原位形成银纳米结构(HORIBA Scientific DeltaDiode和DynaMyc)。

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