利用基因编辑技术修改小鼠基因

Amr R. Salem, Xiaoling Xie, Susan H. Griffin, Lin Gan, Joseph M Miano
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引用次数: 0

摘要

对小鼠进行基因改造,传统上涉及设计和验证靶向构建体、胚胎干细胞电穿孔和选择、囊胚注射以及培育种系传递嵌合体等复杂方法。这些艰巨的步骤最好由学术界专门的基因打靶中心或昂贵的商业供应商来完成。此外,一个项目从启动到完成往往需要至少一年的时间,在某些情况下甚至需要更长的时间(或永远无法完成),而且无法保证成功。RNA 可编程 CRISPR 基因编辑系统大大简化了小鼠基因修饰(如小的替换、插入和缺失)的生成过程,而且成功率很高。目前有几种编辑平台可用于小鼠和其他动物模型的基因/基因组靶向,而在以前很难或根本不可能改变这些基因/基因组。在此,我们提供了一种使用 prime 编辑平台生成转基因小鼠的简化方法。© 2024 Wiley Periodicals LLC.基本方案 1:设计、克隆和合成工程化 pegRNA (epegRNA)基本方案 2:将 PE2 成分显微注射到小鼠子代基本方案 3:基因分型创始小鼠和种系传播育种
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Genetic Modification of Mice Using Prime Editing

Genetically modifying mice traditionally involved complex methods of designing and validating targeting constructs, embryonic stem cell electroporation and selection, blastocyst injection, and breeding chimeras for germline transmission. Such arduous steps were best carried out by specialized gene targeting cores in academia or through expensive commercial vendors. Further, the time from initiation to completion of a project often took at least 1 year and, in some cases, much longer (or never), with no guarantees of success. The RNA-programmable CRISPR system of gene editing has greatly streamlined the generation of gene modifications (e.g., small substitutions, insertions, and deletions) in the mouse with high rates of success. Several editing platforms exist for gene/genome targeting in mice and other animal models previously difficult or impossible to alter. Here, we provide a simplified method of generating genetically modified mice using the prime editing platform. © 2024 Wiley Periodicals LLC.

Basic Protocol 1: Design, cloning, and synthesis of engineered pegRNA (epegRNA)

Basic Protocol 2: Microinjection of PE2 components into mouse zygote

Basic Protocol 3: Genotyping founder mice and breeding for germline transmission

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