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首页> 外文期刊>Methods: A Companion to Methods in Enzymology >Fishing for understanding: Unlocking the zebrafish gene editor's toolbox
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Fishing for understanding: Unlocking the zebrafish gene editor's toolbox

机译:钓鱼理解:解锁Zebrafish Gene编辑器的工具箱

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摘要

The rapid growth of the field of gene editing can largely be attributed to the discovery and optimization of designer endonucleases. These include zinc finger nucleases (ZFNs), transcription activator-like effector nucleases (TALENs), and clustered regular interspersed short palindromic repeat (CRISPR) systems including Cas9, Cas12a, and structure-guided nucleases. Zebrafish (Danio rerio) have proven to be a powerful model system for genome engineering testing and applications due to their external development, high fecundity, and ease of housing. As the zebrafish gene editing toolkit continues to grow, it is becoming increasingly important to understand when and how to utilize which of these technologies for maximum efficacy in a particular project. While CRISPR-Cas9 has brought broad attention to the field of genome engineering in recent years, designer endonucleases have been utilized in genome engineering for more than two decades. This chapter provides a brief overview of designer endonuclease and other gene editing technologies in zebrafish as well as some of their known functional benefits and limitations depending on specific project goals. Finally, selected prospects for additional gene editing tools are presented, promising additional options for directed genomic programming of this versatile animal model system.
机译:基因编辑领域的快速生长可以很大程谷归因于设计者内切核酸酶的发现和优化。这些包括锌手指核酸酶(ZFN),转录活化剂样效应核酸酶(TALENS),并聚集常规穿插短文化重复(CRISPR)系统,包括CAS9,CAS12a和结构引导的核酸酶。由于其外部开发,高繁殖力和容易容易,已证明斑马鱼(Danio Rerio)已被证明是基因组工程测试和应用的强大模型系统。随着斑马鱼基因编辑工具包继续增长,了解何时以及如何利用这些技术在特定项目中的最大效能中越来越重要。虽然CRISPR-CAS9近年来,CASPR-CAS9带来了广泛的关注基因组工程领域,但设计师内切核酸酶已在基因组工程中超过二十年。本章简要概述了设计师内切核酸酶和斑马鱼中的其他基因编辑技术以及他们的一些已知的功能效益和限制,具体取决于具体的项目目标。最后,提出了用于额外基因编辑工具的选定前景,对该多功能动物模型系统的定向基因组编程有前途提供额外的选择。

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