首页> 美国卫生研究院文献>Journal of Visualized Experiments : JoVE >Analyzing In Vivo Cell Migration using Cell Transplantations and Time-lapse Imaging in Zebrafish Embryos
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Analyzing In Vivo Cell Migration using Cell Transplantations and Time-lapse Imaging in Zebrafish Embryos

机译:使用细胞移植和定时成像在斑马鱼胚胎中分析体内细胞迁移。

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摘要

Cell migration is key to many physiological and pathological conditions, including cancer metastasis. The cellular and molecular bases of cell migration have been thoroughly analyzed in vitro. However, in vivo cell migration somehow differs from in vitro migration, and has proven more difficult to analyze, being less accessible to direct observation and manipulation. This protocol uses the migration of the prospective prechordal plate in the early zebrafish embryo as a model system to study the function of candidate genes in cell migration. Prechordal plate progenitors form a group of cells which, during gastrulation, undergoes a directed migration from the embryonic organizer to the animal pole of the embryo. The proposed protocol uses cell transplantation to create mosaic embryos. This offers the combined advantages of labeling isolated cells, which is key to good imaging, and of limiting gain/loss of function effects to the observed cells, hence ensuring cell-autonomous effects. We describe here how we assessed the function of the TORC2 component Sin1 in cell migration, but the protocol can be used to analyze the function of any candidate gene in controlling cell migration in vivo.
机译:细胞迁移是许多生理和病理状况(包括癌症转移)的关键。细胞迁移的细胞和分子基础已在体外进行了全面分析。但是,体内细胞迁移在某种程度上不同于体外迁移,并且已证明更难分析,直接观察和操作较难。该协议使用斑马鱼早期胚胎中前瞻性前庭板的迁移作为模型系统来研究候选基因在细胞迁移中的功能。脊索前板祖细胞形成一组细胞,这些细胞在胃形成过程中经历从胚胎组织者到胚胎动物极的定向迁移。拟议的协议使用细胞移植来创建镶嵌胚胎。这提供了标记分离的细胞的综合优势,这是良好成像的关键,并且可以限制功能效应对观察到的细胞的增减,从而确保了细胞自主效应。我们在这里描述了我们如何评估TORC2组件Sin1在细胞迁移中的功能,但是该协议可用于分析任何候选基因在体内控制细胞迁移的功能。

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