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首页> 外文期刊>Biophysical Journal >Detecting protein complexes in living cells from laser scanning confocal image sequences by the cross correlation raster image spectroscopy method.
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Detecting protein complexes in living cells from laser scanning confocal image sequences by the cross correlation raster image spectroscopy method.

机译:通过互相关光栅图像光谱法从激光扫描共聚焦图像序列检测活细胞中的蛋白质复合物。

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摘要

We describe a general method for detecting molecular complexes based on the analysis of single molecule fluorescence fluctuations from laser scanning confocal images. The method detects and quantifies complexes of two different fluorescent proteins noninvasively in living cells. Because in a raster scanned image successive pixels are measured at different times, the spatial correlation of the image contains information about dynamic processes occurring over a large time range, from the microseconds to seconds. The correlation of intensity fluctuations measured simultaneously in two channels detects protein complexes that carry two molecules of different colors. This information is obtained from the entire image. A map of the spatial distribution of protein complexes in the cell and their diffusion and/or binding properties can be constructed. Using this cross correlation raster image spectroscopy method, specific locations in the cell can be visualized where dynamics of binding and unbinding of fluorescent protein complexes occur. This fluctuation imaging method can be applied to commercial laser scanning microscopes thereby making it accessible to a large community of scientists.
机译:我们描述了一种基于从激光扫描共聚焦图像分析单分子荧光波动来检测分子复合物的一般方法。该方法在活细胞中非侵入性地检测和定量两种不同荧光蛋白的复合物。因为在光栅扫描图像中,连续像素是在不同时间测量的,所以图像的空间相关性包含有关在很大的时间范围(从微秒到秒)内发生的动态过程的信息。在两个通道中同时测量的强度波动的相关性可检测到带有两个不同颜色分子的蛋白质复合物。该信息是从整个图像中获得的。可以构建蛋白质复合物在细胞中的空间分布及其扩散和/或结合特性的图。使用这种互相关光栅图像光谱法,可以观察到细胞中特定位置,在这些位置上发生了荧光蛋白复合物结合和不结合的动力学。这种波动成像方法可以应用于商业激光扫描显微镜,从而使广大的科学家都可以使用。

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