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A high-throughput functional genomics workflow based on CRISPR/Cas9-mediated targeted mutagenesis in zebrafish

机译:基于CRISPR / Cas9介导的斑马鱼靶向诱变的高通量功能基因组学工作流程

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摘要

The zebrafish is a popular model organism for studying development and disease, and genetically modified zebrafish provide an essential tool for functional genomic studies. Numerous publications have demonstrated the efficacy of gene targeting in zebrafish using CRISPR/Cas9, and they have included descriptions of a variety of tools and methods for guide RNA synthesis and mutant identification. However, most of the published techniques are not readily scalable to increase throughput. We recently described a CRISPR/Cas9-based high-throughput mutagenesis and phenotyping pipeline in zebrafish. Here, we present a complete workflow for this pipeline, including target selection; cloning-free single-guide RNA (sgRNA) synthesis; microinjection; validation of the target-specific activity of the sgRNAs; founder screening to identify germline-transmitting mutations by fluorescence PCR; determination of the exact lesion by Sanger or next-generation sequencing (including software for analysis); and genotyping in the F-1 or subsequent generations. Using these methods, sgRNAs can be evaluated in 3 d, zebrafish germline-transmitting mutations can be identified within 3 months and stable lines can be established within 6 months. Realistically, two researchers can target tens to hundreds of genes per year using this protocol.
机译:斑马鱼是研究发育和疾病的流行模型生物,而转基因斑马鱼为功能基因组研究提供了必不可少的工具。许多出版物已经证明了使用CRISPR / Cas9在斑马鱼中靶向基因的功效,并且它们包括了指导RNA合成和突变体鉴定的各种工具和方法的描述。但是,大多数已发布的技术都不容易扩展以增加吞吐量。我们最近在斑马鱼中描述了基于CRISPR / Cas9的高通量诱变和表型传递途径。在这里,我们为该管道提供了完整的工作流程,包括目标选择。无克隆单向导RNA(sgRNA)合成;显微注射验证sgRNA的靶标特异性活性;建立者筛选,通过荧光PCR鉴定种系传递突变;通过Sanger或下一代测序(包括分析软件)确定确切的病变;和F-1或后代的基因分型。使用这些方法,可以在3天内评估sgRNA,可以在3个月内鉴定出传递斑马鱼种系的突变,并可以在6个月内建立稳定的品系。实际上,使用此协议,两名研究人员每年可以靶向数十至数百个基因。

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