TALEN在果蝇诱变和筛选中的优化应用。

Cellular logistics Pub Date : 2015-02-27 eCollection Date: 2015-01-01 DOI:10.1080/21592799.2015.1023423
Han B Lee, Zachary L Sebo, Ying Peng, Yi Guo
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引用次数: 11

摘要

转录激活因子样效应核酸酶(TALENs)已成为基因座特异性基因组工程的有力工具。由于TALEN易于组装,简化TALEN诱导突变的关键在于识别有效的TALEN对并优化TALEN mRNA注射浓度,以最大限度地减少筛选突变后代的工作量。在这里,我们提出了一种简单的方法来定量评估双等位基因的TALEN切割,以及允许精确测量黑腹果蝇体细胞和种系突变率的方法。我们报告说,将候选TALEN mrna先导注射到无Lig4胚胎中的致死率百分比可以用来有效地衡量双等位基因TALEN切割效率,并且以剂量依赖的方式发生。这种及时的lig4依赖性胚胎存活测定也适用于CRISPR/ cas9介导的靶向。此外,利用SURVEYOR核酸酶和毛细管电泳可以快速定量测定G0个体的体细胞突变率,并通过对G0异交后代进行评分来确定种系传播率。总之,这些优化的方法为苍蝇中talen介导的常规基因编辑提供了有效的分步指导。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

An optimized TALEN application for mutagenesis and screening in <i>Drosophila melanogaster</i>.

An optimized TALEN application for mutagenesis and screening in <i>Drosophila melanogaster</i>.

An optimized TALEN application for mutagenesis and screening in <i>Drosophila melanogaster</i>.

An optimized TALEN application for mutagenesis and screening in Drosophila melanogaster.

Transcription activator-like effector nucleases (TALENs) emerged as powerful tools for locus-specific genome engineering. Due to the ease of TALEN assembly, the key to streamlining TALEN-induced mutagenesis lies in identifying efficient TALEN pairs and optimizing TALEN mRNA injection concentrations to minimize the effort to screen for mutant offspring. Here we present a simple methodology to quantitatively assess bi-allelic TALEN cutting, as well as approaches that permit accurate measures of somatic and germline mutation rates in Drosophila melanogaster. We report that percent lethality from pilot injection of candidate TALEN mRNAs into Lig4 null embryos can be used to effectively gauge bi-allelic TALEN cutting efficiency and occurs in a dose-dependent manner. This timely Lig4-dependent embryonic survival assay also applies to CRISPR/Cas9-mediated targeting. Moreover, the somatic mutation rate of individual G0 flies can be rapidly quantitated using SURVEYOR nuclease and capillary electrophoresis, and germline transmission rate determined by scoring progeny of G0 outcrosses. Together, these optimized methods provide an effective step-wise guide for routine TALEN-mediated gene editing in the fly.

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