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Increasing the Targeting Scope of CRISPR Base Editing System Beyond NGG

机译:增加针对CRISPR基地的范围编辑系统NGG之外

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摘要

Genome editing provides a new therapeutic strategy to cure genetic diseases. The recently developed CRISPR-Cas9 base editing technology has shown great potential to repair the majority of pathogenic point mutations in the patient's DNA precisely. Base editor is the fusion of a Cas9 nickase with a base-modifying enzyme that can change a nucleotide on a single strand of DNA without generating double-stranded DNA breaks. However, a major limitation in applying such a system is the prerequisite of a protospacer adjacent motif sequence at the desired position relative to the target site. Progress has been made to increase the targeting scope of base editors by engineering SpCas9 protein variants, establishing systems with broadened editing windows, characterizing new SpCas9 orthologs, and developing prime editing technology. In this review, we discuss recent progress in the development of CRISPR base editing, focusing on its targeting scope, and we provide a workflow for selecting a suitable base editor based on the target nucleotide sequences.
机译:基因组编辑提供了一种新的治疗策略治疗遗传性疾病。编辑技术显示CRISPR-Cas9基地巨大的潜力来修复的大部分致病性点突变在病人的DNA精确。nickase base-modifying酶,这种酶可以改变一个核苷酸单链的DNA没有生成双链DNA断裂。然而,一个主要限制在应用这样一个系统是protospacer的先决条件相邻的主题序列在所需的位置相对于目标站点。增加基础的目标范围编辑通过工程SpCas9蛋白变体,建立与扩大编辑系统窗户,描述新的SpCas9直接同源'编辑技术发展。审查,我们将讨论最近的进展编辑CRISPR基地的发展,关注其目标范围,我们提供一个工作流编辑器的基础上,选择一个合适的基地目标核苷酸序列。

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