Chemical Biology Approaches to Genome Editing: Understanding, Controlling, and Delivering Programmable Nucleases

基因组编辑 转录激活物样效应核酸酶 清脆的 基因组工程 生物 Cas9 计算生物学 锌指核酸酶 效应器 基因组 DNA 合成生物学 劈开 核酸酶 遗传学 基因 细胞生物学
作者
Johnny H. Hu,Kevin M Davis,David R. Liu
出处
期刊:Cell chemical biology [Elsevier]
卷期号:23 (1): 57-73 被引量:41
标识
DOI:10.1016/j.chembiol.2015.12.009
摘要

Programmable DNA nucleases have provided scientists with the unprecedented ability to probe, regulate, and manipulate the human genome. Zinc-finger nucleases (ZFNs), transcription activator-like effector nucleases (TALENs), and the clustered regularly interspaced short palindromic repeat-Cas9 system (CRISPR-Cas9) represent a powerful array of tools that can bind to and cleave a specified DNA sequence. In their canonical forms, these nucleases induce double-strand breaks at a DNA locus of interest that can trigger cellular DNA repair processes that disrupt or replace genes. The fusion of these programmable nucleases with a variety of other protein domains has led to a rapidly growing suite of tools for activating, repressing, visualizing, and modifying loci of interest. Maximizing the usefulness and therapeutic relevance of these tools, however, requires precisely controlling their activity and specificity to minimize potentially toxic side effects arising from off-target activities. This need has motivated the application of chemical biology principles and methods to genome-editing proteins, including the engineering of variants of these proteins with improved or altered specificities, and the development of genetic, chemical, optical, and protein delivery methods that control the activity of these agents in cells. Advancing the capabilities, safety, effectiveness, and therapeutic relevance of genome-engineering proteins will continue to rely on chemical biology strategies that manipulate their activity, specificity, and localization.

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