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Combined use of in ovo electroporation and cultured neurons for gene function analysis of embryogenesis in the chicken optic tectum

机译:在鸡视窗中胚胎电穿孔和培养神经元的结合使用在鸡视窗中胚胎发生的基因功能分析

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Chicken embryos are used widely in the fields of developmental biology and neurobiology. The chicken embryo also serves as a model to analyze gene expression and function using in ovo electroporation. Plasmids may be injected into the spinal cord or tectum of the chicken central nervous system by microinjection for electroporation. Here, we developed a novel method that combines in ovo electroporation and neuronal culturing to study gene function in the chicken tectum during embryo development. Our method can be used to study in-vivo and in-vitro exogenous genes' function. In addition, live cell imaging microscopy, immunostaining, and transfection can be used with our method to study neuronal growth, development, neurite growth and retraction, and axonal pathfinding. Our result showed that axons were present in isolated neurons after culturing for 24 h, and cell debris was low after replacing the media at 48 h. Many GFP-expressing neurons were observed in the cultured cells after 48 h. We successfully cultured the neurons for 3 weeks. Together, this method combines in ovo electroporation and neuronal culturing advantages and is more convenient for the gene function analysis. Copyright (C) 2017 Wolters Kluwer Health, Inc. All rights reserved.
机译:鸡胚胎广泛用于发育生物学和神经生物学领域。鸡胚还用作分析基因表达和使用在卵oO电穿孔的模型。通过显微注射用于电穿孔,可以将质粒注射到鸡中枢神经系统的脊髓或构图中。在这里,我们开发了一种新的方法,其在胚胎发育期间将卵泡电穿孔和神经元培养结合在鸡胶中研究基因功能。我们的方法可用于研究体内和体外外源基因的功能。此外,实时细胞成像显微镜,免疫染色和转染可以与我们研究神经元生长,发育,神经突生长和缩回和轴突探测器的方法一起使用。我们的结果表明,在培养24小时后,轴突出现在培养后,在48小时后置换培养基后,细胞碎片低。在48小时后在培养的细胞中观察到许多GFP表达神经元。我们成功培养了神经元3周。这种方法在一起结合在卵子电穿孔和神经元培养优势中,对基因功能分析更方便。版权所有(C)2017 Wolters Kluwer Health,Inc。保留所有权利。

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