首页> 外文期刊>Developmental dynamics: an official publication of the American Association of Anatomists >Imaging brain development and organogenesis in zebrafish using immobilized embryonic explants.
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Imaging brain development and organogenesis in zebrafish using immobilized embryonic explants.

机译:使用固定的胚胎外植体成像斑马鱼的大脑发育和器官发生。

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Owing to its optical clarity and rapid rate of development, the zebrafish embryo is an ideal model system for studying the cellular mechanics of organogenesis. Unfortunately, extended time-lapse recordings of zebrafish embryos are often disrupted by the extension and straightening of the embryonic axis, as well as movement artifacts associated with developing musculature. In addition, the embryo's massive yolk cell often prevents optical access to tissues of interest. To circumvent these imaging problems, we have developed a procedure to deflate and mechanically remove the yolk cell. A "paralyzing" agent, AMP-PNP (a membrane-impermeant nonhydrolyzable analog of ATP), is first injected into the embryo's contractile yolk cell. The yolk cell is then removed using sharpened tungsten needles. Deyolked embryos, or organ rudiments explanted from them, are then immobilized on a microscope coverslip using a thin plasma clot. This plasma clot immobilization allows novel mountings of the explants so that ventral,lateral, and even cross-sectional fields of views are possible using high numerical aperture objectives. We show that isolated head rudiments undergo normal morphogenesis and gene expression for at least 1 day after being explanted into organotypic culture. These procedures can be used to study the cellular mechanics of organogenesis in deyolked protein transgenic animals. Developmental Dynamics 2003.
机译:由于其光学清晰度和快速发展速度,斑马鱼胚胎是研究器官发生的细胞力学的理想模型系统。不幸的是,斑马鱼胚胎的延时记录经常会因胚胎轴的延伸和拉直以及与肌肉组织发展相关的运动伪影而中断。此外,胚胎的卵黄细胞通常会阻止光学途径进入目标组织。为了规避这些成像问题,我们开发了一种程序来放气并机械去除卵黄细胞。首先将“麻痹”剂AMP-PNP(ATP的膜不渗透性不可水解类似物)注射到胚胎的收缩卵黄细胞中。然后使用尖锐的钨针去除卵黄细胞。然后,使用稀薄的血浆凝块将脱液的胚胎或从中取出的器官残基固定在显微镜盖玻片上。这种血浆凝块的固定允许外植体的新颖安装,从而可以使用高数值孔径的物镜来实现腹面,侧面甚至横截面的视野。我们显示,孤立的头小伙子移植到器官型文化后至少经历1天的正常形态发生和基因表达。这些程序可用于研究脱脂蛋白转基因动物器官发生的细胞机制。开发动力学2003。

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