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Calibration of fluorescence resonance energy transfer in microscopy

机译:显微镜下荧光共振能量转移的校准

摘要

Imaging hardware, software, calibrants, and methods are provided to visualize and quantitate the amount of Fluorescence Resonance Energy Transfer (FRET) occurring between donor and acceptor molecules in epifluorescence microscopy. The MicroFRET system compensates for overlap among donor, acceptor, and FRET spectra using well characterized fluorescent beads as standards in conjunction with radiometrically calibrated image processing techniques. The MicroFRET system also provides precisely machined epifluorescence cubes to maintain proper image registration as the sample is illuminated at the donor and acceptor excitation wavelengths. Algorithms are described that pseudocolor the image to display pixels exhibiting radiometrically-corrected fluorescence emission from the donor (blue), the acceptor (green) and FRET (red). The method is demonstrated on samples exhibiting FRET between genetically engineered derivatives of the Green Fluorescent Protein (GFP) bound to the surface of Ni chelating beads by histidine-tags.
机译:提供了成像硬件,软件,校准物和方法,以可视化和量化落射荧光显微镜中供体分子和受体分子之间发生的荧光共振能量转移(FRET)的数量。 MicroFRET系统使用特征明确的荧光珠作为标准,结合辐射校准的图像处理技术,补偿供体,受体和FRET光谱之间的重叠。 MicroFRET系统还提供经过精确加工的落射荧光立方体,以在以供体和受体激发波长照射样品时保持适当的图像配准。描述了对图像进行伪彩色以显示像素的像素的算法,这些像素显示出来自供体(蓝色),受体(绿色)和FRET(红色)的经辐射校正的荧光发射。在通过组氨酸标签结合到Ni螯合微珠表面的绿色荧光蛋白(GFP)的基因工程衍生物之间表现出FRET的样品上证实了该方法。

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