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Gene application with in utero electroporation in mouse embryonic brain

机译:基因在小鼠胚胎脑子宫电穿孔中的应用

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Mouse genetic manipulations, such as the production of gene knock-out, knock-in, and transgenic mice, have provided excellent systems for analysis of numerous genes functioning during development. Nevertheless, the lack of specific promoters and enhancers that control gene expression in specific regions and at specific times, limits usage of these techniques. However, progress in in utero systems of electroporation into mouse embryos has opened a new window, permitting new approaches to answering important questions. Simple injection of plasmid DNA solution and application of electrical current to mouse embryos results in transient area- and time-dependent transfection. Further modification of the technique, arising from variations in types of electrodes used, has made it possible to control the relative size of the region of transfection, which can vary from a few cells to entire tissues. Thus, this technique is a powerful means not only of characterizing gene function in various settings, but also of tracing the migratory routes of cells, due to its high efficiency and the localization of gene expression it yields. We summarize here some of the potential uses and advantages of this technique for developmental neuroscience research.
机译:小鼠基因操作,例如基因敲除,敲入和转基因小鼠的产生,为分析发育过程中众多功能基因提供了出色的系统。然而,缺乏控制特定区域和特定时间的基因表达的特异性启动子和增强子,限制了这些技术的使用。但是,子宫内电穿孔进入小鼠胚胎的子宫内系统的进步打开了一个新的窗口,为回答重要问题提供了新的方法。简单注射质粒DNA溶液并将电流施加到小鼠胚胎会导致瞬时的区域和时间依赖性转染。由于所用电极类型的变化而引起的对该技术的进一步修改,使得可以控制转染区域的相对大小,该相对大小可以从几个细胞到整个组织变化。因此,由于它的高效率和它产生的基因表达的定位,该技术不仅是表征各种环境中基因功能的有力手段,而且是追踪细胞迁移途径的有力手段。我们在这里总结了该技术在发展神经科学研究中的一些潜在用途和优点。

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