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CRISPR/Cas Systems in Genome Editing: Methodologies and Tools for sgRNA Design Off‐Target Evaluation and Strategies to Mitigate Off‐Target Effects

机译:基因组编辑中的CRISPR / Cas系统:sgRNA设计脱靶评估和缓解脱靶效应的策略的方法和工具

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摘要

Life sciences have been revolutionized by genome editing (GE) tools, including zinc finger nucleases, transcription activator‐Like effector nucleases, and CRISPR (clustered regulatory interspaced short palindromic repeats)/Cas (CRISPR‐associated) systems, which make the targeted modification of genomic DNA of all organisms possible. CRISPR/Cas systems are being widely used because of their accuracy, efficiency, and cost‐effectiveness. Various classes of CRISPR/Cas systems have been developed, but their extensive use may be hindered by off‐target effects. Efforts are being made to reduce the off‐target effects of CRISPR/Cas9 by generating various CRISPR/Cas systems with high fidelity and accuracy. Several approaches have been applied to detect and evaluate the off‐target effects. Here, the current GE tools, the off‐target effects generated by GE technology, types of off‐target effects, mechanisms of off‐target effects, major concerns, and outcomes of off‐target effects in plants and animals are summarized. The methods to detect off‐target effects, tools for single‐guide RNA (sgRNA) design, evaluation and prediction of off‐target effects, and strategies to increase the on‐target efficiency and mitigate the off‐target impact on intended genome‐editing outcomes are summarized.
机译:生命科学已经通过基因组编辑(GE)工具进行了革新,包括锌指核酸酶,转录激活子样效应子核酸酶和CRISPR(聚类调控间隔短回文重复序列)/ Cas(CRISPR相关)系统,可对所有生物的基因组DNA都是可能的。 CRISPR / Cas系统由于其准确性,效率和成本效益而被广泛使用。已经开发了各种类型的CRISPR / Cas系统,但脱靶效应可能会阻碍其广泛使用。人们正在努力通过生成各种具有高保真度和准确性的CRISPR / Cas系统来减少CRISPR / Cas9的脱靶效应。已经应用了几种方法来检测和评估脱靶效应。在这里,总结了当前的GE工具,GE技术产生的脱靶效应,脱靶效应的类型,脱靶效应的机制,主要问题以及动植物的脱靶效应的结果。检测脱靶效应的方法,单向导RNA(sgRNA)设计工具,脱靶效应的评估和预测,以及提高脱靶效率和减轻脱靶对预期基因组编辑影响的策略结果总结。

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