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Practical guide of live imaging for developmental biologists

机译:发育生物学家实时成像实用指南

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Time-lapse imaging of fluorescent proteins in living cells has become an indispensable tool in biological sciences. However, its application at the organismal level still faces a number of obstacles, such as large specimen sizes preventing illumination of internal tissues, high background fluorescence and uncontrollable movement of target tissues or embryos. Here we describe our solutions for these issues to obtain 4-D fluorescent images from living Drosophila embryos using confocal microscopes. A computational procedure that detects and corrects the shift of moving objects to virtually stabilize them in time-lapse movies (iSEMS) is presented. We discuss the importance of postimaging treatment of raw image stacks for the discovery of novel phenotypes that have previously escaped attention from the analyses of fixed specimens.
机译:活细胞中荧光蛋白的延时成像已成为生物科学中必不可少的工具。但是,其在生物体水平的应用仍然面临许多障碍,例如大样本尺寸会阻止内部组织的照明,高背景荧光以及目标组织或胚胎的无法控制的运动。在这里,我们描述了针对这些问题的解决方案,以使用共聚焦显微镜从果蝇活体胚胎中获得4-D荧光图像。提出了一种计算程序,该程序可以检测并校正移动物体的移动,以使它们在延时电影(iSEMS)中几乎稳定下来。我们讨论原始图像堆栈的后成像处理对于发现新表型的重要性,这些新表型先前已从固定标本的分析中引起关注。

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