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利用 TALEN 技术在小鼠中进行高效靶向诱变。

Highly efficient targeted mutagenesis in mice using TALENs.

机构信息

Institute of Developmental Genetics, Helmholtz Zentrum München, German Research Center for Environmental Health, 85764 Munich, Germany.

出版信息

Genetics. 2013 Nov;195(3):703-13. doi: 10.1534/genetics.113.156570. Epub 2013 Aug 26.

Abstract

Targeted mouse mutants are instrumental for the analysis of gene function in health and disease. We recently provided proof-of-principle for the fast-track mutagenesis of the mouse genome, using transcription activator-like effector nucleases (TALENs) in one-cell embryos. Here we report a routine procedure for the efficient production of disease-related knockin and knockout mutants, using improved TALEN mRNAs that include a plasmid-coded poly(A) tail (TALEN-95A), circumventing the problematic in vitro polyadenylation step. To knock out the C9orf72 gene as a model of frontotemporal lobar degeneration, TALEN-95A mutagenesis induced sequence deletions in 41% of pups derived from microinjected embryos. Using TALENs together with mutagenic oligodeoxynucleotides, we introduced amyotrophic lateral sclerosis patient-derived missense mutations in the fused in sarcoma (Fus) gene at a rate of 6.8%. For the simple identification of TALEN-induced mutants and their progeny we validate high-resolution melt analysis (HRMA) of PCR products as a sensitive and universal genotyping tool. Furthermore, HRMA of off-target sites in mutant founder mice revealed no evidence for undesired TALEN-mediated processing of related genomic sequences. The combination of TALEN-95A mRNAs for enhanced mutagenesis and of HRMA for simplified genotyping enables the accelerated, routine production of new mouse models for the study of genetic disease mechanisms.

摘要

靶向鼠突变体是分析健康和疾病相关基因功能的重要工具。我们最近使用转录激活因子样效应物核酸酶(TALENs)在单细胞胚胎中证明了快速突变鼠基因组的原理。在这里,我们报告了一种使用改良的 TALEN mRNA 高效生产与疾病相关的基因敲入和敲除突变体的常规程序,该改良的 TALEN mRNA 包含质粒编码的 poly(A)尾(TALEN-95A),绕过了有问题的体外多聚腺苷酸化步骤。为了敲除 C9orf72 基因作为额颞叶变性的模型,TALEN-95A 诱变在源自微注射胚胎的 41%的幼鼠中诱导了序列缺失。使用 TALEN 与诱变寡脱氧核苷酸,我们以 6.8%的效率在融合肉瘤(Fus)基因中引入了肌萎缩侧索硬化症患者来源的错义突变。为了简单地鉴定 TALEN 诱导的突变体及其后代,我们验证了 PCR 产物的高分辨率熔解分析(HRMA)作为一种敏感和通用的基因分型工具。此外,突变体创始鼠中靶外位点的 HRMA 未显示出 TALEN 介导的相关基因组序列处理的不良证据。TALEN-95A mRNA 用于增强诱变和 HRMA 用于简化基因分型的组合使新的遗传疾病机制研究的小鼠模型的加速常规生产成为可能。

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