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利用简化的 CRISPR/Cas9 基因敲入方法在斑马鱼中进行内源性蛋白标记。

Endogenous protein tagging in medaka using a simplified CRISPR/Cas9 knock-in approach.

机构信息

Developmental Biology Unit, European Molecular Biology Laboratory, Heidelberg, Germany.

出版信息

Elife. 2021 Dec 6;10:e75050. doi: 10.7554/eLife.75050.

Abstract

The CRISPR/Cas9 system has been used to generate fluorescently labelled fusion proteins by homology-directed repair in a variety of species. Despite its revolutionary success, there remains an urgent need for increased simplicity and efficiency of genome editing in research organisms. Here, we establish a simplified, highly efficient, and precise strategy for CRISPR/Cas9-mediated endogenous protein tagging in medaka (). We use a cloning-free approach that relies on PCR-amplified donor fragments containing the fluorescent reporter sequences flanked by short homology arms (30-40 bp), a synthetic single-guide RNA and Cas9 mRNA. We generate eight novel knock-in lines with high efficiency of F0 targeting and germline transmission. Whole genome sequencing results reveal single-copy integration events only at the targeted . We provide an initial characterization of these fusion protein lines, significantly expanding the repertoire of genetic tools available in medaka. In particular, we show that the line has the potential to serve as an organismal-wide label for proliferative zones and an endogenous cell cycle reporter.

摘要

CRISPR/Cas9 系统已被用于通过同源定向修复在多种物种中生成荧光标记的融合蛋白。尽管它取得了革命性的成功,但在研究生物中,仍然迫切需要提高基因组编辑的简单性和效率。在这里,我们建立了一种简化、高效、精确的 CRISPR/Cas9 介导的鱼类内源蛋白标记策略()。我们使用一种无克隆的方法,该方法依赖于包含荧光报告序列的 PCR 扩增供体片段,侧翼是短同源臂(30-40bp)、合成的单指导 RNA 和 Cas9 mRNA。我们以高效率的 F0 靶向和种系传递生成了八个新的敲入系。全基因组测序结果仅在靶向的 处显示单拷贝整合事件。我们对这些融合蛋白系进行了初步表征,显著扩展了鱼类中可用的遗传工具库。特别是,我们表明 系有可能成为增殖区的全器官标记物和内源性细胞周期报告基因。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a3b8/8691840/33924da152b8/elife-75050-fig1.jpg

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