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Live Imaging of the Zebrafish Embryonic Brain by Confocal Microscopy

机译:共聚焦显微镜对斑马鱼胚胎脑的实时成像

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摘要

In this video, we demonstrate the method our lab has developed to analyze the cell shape changes and rearrangements required to bend and fold the developing zebrafish brain (Gutzman et al, 2008). Such analysis affords a new understanding of the underlying cell biology required for development of the 3D structure of the vertebrate brain, and significantly increases our ability to study neural tube morphogenesis. The embryonic zebrafish brain is shaped beginning at 18 hours post fertilization (hpf) as the ventricles within the neuroepithelium inflate. By 24 hpf, the initial steps of neural tube morphogenesis are complete. Using the method described here, embryos at the one cell stage are injected with mRNA encoding membrane-targeted green fluorescent protein (memGFP). After injection and incubation, the embryo, now between 18 and 24 hpf, is mounted, inverted, in agarose and imaged by confocal microscopy. Notably, the zebrafish embryo is transparent making it an ideal system for fluorescent imaging. While our analyses have focused on the midbrain-hindbrain boundary and the hindbrain, this method could be extended for analysis of any region in the zebrafish to a depth of 80-100 μm.
机译:在此视频中,我们演示了实验室开发的用于分析弯曲和折叠发育中的斑马鱼大脑所需的细胞形状变化和重排的方法(Gutzman等,2008)。此类分析为开发脊椎动物大脑3D结构所需的基础细胞生物学提供了新的认识,并显着提高了我们研究神经管形态发生的能力。斑马鱼胚胎的大脑在受精(hpf)后18小时开始成形,因为神经上皮内的心室膨胀。到24 hpf,神经管形态发生的初始步骤已完成。使用此处描述的方法,在一个细胞阶段的胚胎中注入编码膜靶向绿色荧光蛋白(memGFP)的mRNA。注射和孵育后,将现在处于18和24 hpf之间的胚胎装入琼脂糖中,倒置,并用共聚焦显微镜成像。值得注意的是,斑马鱼的胚胎是透明的,使其成为荧光成像的理想系统。虽然我们的分析集中在中脑-后脑边界和后脑,但该方法可以扩展到斑马鱼中任何区域的分析,深度为80-100μm。

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