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用于转染以及活细胞和亚细胞成像的斑马鱼胚胎原代细胞培养。

Embryonic zebrafish primary cell culture for transfection and live cellular and subcellular imaging.

作者信息

Sassen Wiebke A, Lehne Franziska, Russo Giulio, Wargenau Sven, Dübel Stefan, Köster Reinhard W

机构信息

Division of Cellular and Molecular Neurobiology, Zoological Institute, Braunschweig University of Technology, 38106 Braunschweig, Germany.

Division of Cellular and Molecular Neurobiology, Zoological Institute, Braunschweig University of Technology, 38106 Braunschweig, Germany; Department of Biotechnology and Bioinformatics, Braunschweig University of Technology, Braunschweig 38106, Germany.

出版信息

Dev Biol. 2017 Oct 1;430(1):18-31. doi: 10.1016/j.ydbio.2017.07.014. Epub 2017 Aug 9.

Abstract

Although having great potential for live cell imaging to address numerous cell biological questions with high spatial and temporal resolution, primary cell cultures of zebrafish embryos are not widely used. We present an easy-to-use protocol for preparing primary cell cultures of 2 dpf zebrafish embryos allowing for live cell imaging of fully differentiated cells such as neurons and myocytes. We demonstrate that different cell types can be identified by morphology and expression of transgenic cell type-specific fluorescent reporters and that fluorescent cells can be sorted by flow cytometry to prepare an enriched culture. To facilitate subcellular imaging in live primary cells, we successfully tested a selection of fluorescent vital dyes. Most importantly, we demonstrate that zebrafish primary cells can be transfected efficiently with expression constructs allowing for visualizing subcellular structures with fluorescent marker proteins for time lapse imaging. We propose zebrafish primary cell culture as a versatile tool to address cell biological questions in combination with a powerful in vivo model.

摘要

尽管斑马鱼胚胎原代细胞培养在活细胞成像方面具有很大潜力,能够以高空间和时间分辨率解决众多细胞生物学问题,但它并未得到广泛应用。我们提出了一种易于使用的方案,用于制备2天龄斑马鱼胚胎的原代细胞培养物,以便对神经元和心肌细胞等完全分化的细胞进行活细胞成像。我们证明,不同的细胞类型可以通过形态学和转基因细胞类型特异性荧光报告基因的表达来识别,并且荧光细胞可以通过流式细胞术进行分选,以制备富集培养物。为了便于在活原代细胞中进行亚细胞成像,我们成功测试了一系列荧光活性染料。最重要的是,我们证明斑马鱼原代细胞可以用表达构建体高效转染,从而通过荧光标记蛋白可视化亚细胞结构以进行延时成像。我们提出将斑马鱼原代细胞培养作为一种多功能工具,与强大的体内模型相结合来解决细胞生物学问题。

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