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Fluorescence resonance energy transfer (FRET) measurement by gradual acceptor photobleaching.

机译:通过逐步的受体光漂白测量荧光共振能量转移(FRET)。

摘要

Fluorescence resonance energy transfer (FRET) is an extremely effective tool to detect molecular interaction at suboptical resolutions. One of the techniques for measuring FRET is acceptor photobleaching: the increase in donor fluorescence after complete acceptor photobleaching is a measure of the FRET efficiency. However, in wide-field microscopy, complete acceptor photobleaching is difficult due to the low excitation intensities. In addition, the method is sensitive to inadvertent donor bleaching, autofluorescence and bleed-through of excitation light. In the method introduced in this paper, donor and acceptor intensities are monitored continuously during acceptor photobleaching. Subsequently, curve fitting is used to determine the FRET efficiency. The method was demonstrated on cameleon (YC2.1), a FRET-based Ca(2+) indicator, and on a CFP-YFP fusion protein expressed in HeLa cells. FRET efficiency of cameleon in the presence of 1 mm Ca(2+) was 31 +/- 3%. In the absence of Ca(2+) a FRET efficiency of 15 +/- 2% was found. A FRET efficiency of 28% was found for the CFP-YFP fusion protein in HeLa cells. Advantages of the method are that it does not require complete acceptor photobleaching, it includes correction for spectral cross-talk, donor photobleaching and autofluorescence, and is relatively simple to use on a normal wide-field microscope.
机译:荧光共振能量转移(FRET)是检测亚光学分辨率下分子相互作用的极为有效的工具。测量FRET的一种技术是受体光漂白:在完全的受体光漂白之后,供体荧光的增加是FRET效率的量度。但是,在宽视场显微镜中,由于激发强度低,因此很难进行完全的受体光漂白。此外,该方法对疏忽的供体漂白,自发荧光和激发光渗漏敏感。在本文介绍的方法中,在受体光漂白过程中连续监测供体和受体的强度。随后,使用曲线拟合确定FRET效率。该方法在基于FRET的Ca(2+)指示剂cameleon(YC2.1)和在HeLa细胞中表达的CFP-YFP融合蛋白上得到了证明。在1毫米Ca(2+)存在下,喀麦隆的FRET效率为31 +/- 3%。在不存在Ca(2+)的情况下,发现FRET效率为15 +/- 2%。发现HeLa细胞中CFP-YFP融合蛋白的FRET效率为28%。该方法的优点是它不需要完全的受体光漂白,它包括校正光谱串扰,施主光漂白和自发荧光,并且在普通的宽视场显微镜上使用相对简单。

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