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通过微注射到两细胞期小鼠胚胎中高效产生靶向大片段插入。

Efficient generation of targeted large insertions by microinjection into two-cell-stage mouse embryos.

机构信息

Program in Developmental and Stem Cell Biology, Hospital for Sick Children, Toronto, Ontario, Canada.

Department of Molecular Genetics, University of Toronto, Toronto, Ontario, Canada.

出版信息

Nat Biotechnol. 2018 Aug;36(7):632-637. doi: 10.1038/nbt.4166. Epub 2018 Jun 11.

Abstract

Rapid, efficient generation of knock-in mice with targeted large insertions remains a major hurdle in mouse genetics. Here, we describe two-cell homologous recombination (2C-HR)-CRISPR, a highly efficient gene-editing method based on introducing CRISPR reagents into embryos at the two-cell stage, which takes advantage of the open chromatin structure and the likely increase in homologous-recombination efficiency during the long G2 phase. Combining 2C-HR-CRISPR with a modified biotin-streptavidin approach to localize repair templates to target sites, we achieved a more-than-tenfold increase (up to 95%) in knock-in efficiency over standard methods. We targeted 20 endogenous genes expressed in blastocysts with fluorescent reporters and generated reporter mouse lines. We also generated triple-color blastocysts with all three lineages differentially labeled, as well as embryos carrying the two-component auxin-inducible degradation system for probing protein function. We suggest that 2C-HR-CRISPR is superior to random transgenesis or standard genome-editing protocols, because it ensures highly efficient insertions at endogenous loci and defined 'safe harbor' sites.

摘要

快速、高效地生成带有靶向大片段插入的基因敲入小鼠仍然是小鼠遗传学中的一个主要障碍。在这里,我们描述了一种基于在二细胞期将 CRISPR 试剂引入胚胎的高效基因编辑方法——两细胞同源重组 (2C-HR)-CRISPR,该方法利用了开放染色质结构和 G2 期长时可能增加的同源重组效率。将 2C-HR-CRISPR 与改良的生物素-链霉亲和素方法相结合,将修复模板定位到靶位点,我们实现了敲入效率比标准方法提高了十倍以上(高达 95%)。我们用荧光报告基因靶向了囊胚中表达的 20 个内源性基因,并生成了报告基因小鼠系。我们还生成了带有三种谱系差异标记的三色囊胚,以及携带双组分生长素诱导降解系统的胚胎,用于探测蛋白质功能。我们认为 2C-HR-CRISPR 优于随机转基因或标准基因组编辑方案,因为它可以确保在内源性基因座和定义的“安全港”位点高效地进行插入。

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