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利用非洲爪蟾的共聚焦分析研究Wnt和Shh形态发生素梯度的调节因子。

Using Confocal Analysis of Xenopus laevis to Investigate Modulators of Wnt and Shh Morphogen Gradients.

作者信息

Fellgett Simon W, Ramsbottom Simon A, Maguire Richard J, Cross Stephen, O'Toole Peter, Pownall Mary E

机构信息

Department of Biomedical Science, The Bateson Centre, University of Sheffield.

Institute of Genetic Medicine, Newcastle University.

出版信息

J Vis Exp. 2015 Dec 14(106):e53162. doi: 10.3791/53162.

Abstract

This protocol describes a method to visualise ligands distributed across a field of cells. The ease of expressing exogenous proteins, together with the large size of their cells in early embryos, make Xenopus laevis a useful model for visualising GFP-tagged ligands. Synthetic mRNAs are efficiently translated after injection into early stage Xenopus embryos, and injections can be targeted to a single cell. When combined with a lineage tracer such as membrane tethered RFP, the injected cell (and its descendants) that are producing the overexpressed protein can easily be followed. This protocol describes a method for the production of fluorescently tagged Wnt and Shh ligands from injected mRNA. The methods involve the micro dissection of ectodermal explants (animal caps) and the analysis of ligand diffusion in multiple samples. By using confocal imaging, information about ligand secretion and diffusion over a field of cells can be obtained. Statistical analyses of confocal images provide quantitative data on the shape of ligand gradients. These methods may be useful to researchers who want to test the effects of factors that may regulate the shape of morphogen gradients.

摘要

本方案描述了一种可视化分布在细胞群中的配体的方法。易于表达外源蛋白,以及早期胚胎中细胞体积较大,使得非洲爪蟾成为用于可视化绿色荧光蛋白标记配体的有用模型。合成mRNA注射到非洲爪蟾早期胚胎后能有效翻译,并且注射可以靶向单个细胞。当与诸如膜连接的红色荧光蛋白等谱系示踪剂结合使用时,产生过表达蛋白的注射细胞(及其后代)很容易被追踪。本方案描述了一种从注射的mRNA产生荧光标记的Wnt和Shh配体的方法。这些方法包括外胚层外植体(动物帽)的显微解剖以及多个样本中配体扩散的分析。通过使用共聚焦成像,可以获得有关配体在细胞群中分泌和扩散的信息。共聚焦图像的统计分析提供了关于配体梯度形状的定量数据。这些方法可能对想要测试可能调节形态发生素梯度形状的因素的影响的研究人员有用。

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本文引用的文献

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