首页> 外文期刊>Cryobiology: International Journal of Low Temperature Biology and Medicine >Genome editing of rodents by electroporation of CRISPR/Cas9 into frozen-warmed pronuclear-stage embryos
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Genome editing of rodents by electroporation of CRISPR/Cas9 into frozen-warmed pronuclear-stage embryos

机译:通过将CRISPR / CAS9电穿孔进入冷冻温热的强化阶段胚胎的基因组编辑

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摘要

Genome edited animals can now be easily produced using the clustered regularly interspaced short palindromic repeat (CRISPR) and CRISPR-associated protein 9 (Cas9) system. Traditionally, these animals have been produced by the introduction of endonucleases into pronuclear-stage embryos. Recently, a novel electroporation method, the "Technique for Animal Knockout system by Electroporation (TAKE)," has been established as a simple and highly efficient tool to introduce endonucleases into embryos instead of methods such as microinjection. Use of frozen-warmed pronuclear-stage embryos in this method has further contributed to efficient production of genome edited animals. However, early developmental stage embryos, including pronuclear-stage embryos, especially those of rats, sometimes show low resistance to physical damage by vitrification and introduction of endonucleases during microinjection. In this study, we propose an ethanol-free, slow-freezing method to reduce physical damage to pronuclear-stage embryos followed by the TAKE method. All mouse and rat frozen embryos were survived after electroporation, and 18% and 100% of offspring were edited target gene, respectively. The resulting protocol is an efficient method for producing genome edited animals.
机译:基因组编辑的动物现在可以使用聚类定期间隙的短语重复(CRISPR)和CRISPR相关蛋白质9(CAS9)系统来容易地生产。传统上,这些动物已经通过将内切核酸酶引入核核胚胎而产生。最近,一种新型电穿孔方法,“通过电穿孔(采用)的动物淘汰系统技术”,已经建立了一种简单且高效的工具,以将内切核酸酶引入胚胎而不是微注射等方法。在该方法中使用冷冻温热的强核阶段胚胎进一步有助于有效地生产基因组编辑的动物。然而,早期发育阶段胚胎,包括经核胚胎,尤其是大鼠的胚胎,有时会通过玻璃化和引入显微注射期间的内切核酸酶的低抗性。在这项研究中,我们提出了一种无乙醇,缓慢冷冻方法,以减少对核核胚胎的物理损伤,然后采取方法。在电穿孔后存活所有小鼠和大鼠冷冻胚胎,分别编辑了18%和100%的后代靶基因。所得方案是一种产生基因组编辑动物的有效方法。

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