小鼠胚胎中 CRISPR/Cas9 独立于 sgRNA 序列的 DNA 切割的发现与特征。

IF 4.3 3区 材料科学 Q1 ENGINEERING, ELECTRICAL & ELECTRONIC ACS Applied Electronic Materials Pub Date : 2024-03-25 DOI:10.1016/j.ygeno.2024.110836
Liyun Yang , Lijiao Chen , Yang Zheng , Li Deng , Raoxian Bai , Ting Zhang , Zhengbo Wang , Shangang Li
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引用次数: 0

摘要

在程序化基因编辑过程中,CRISPR/Cas9系统可诱发脱靶效应,但有关胚胎发育过程中的裂解检测及其影响的报道却很少。为了研究这些事件,我们设计了不同脱靶率的 sgRNA,将其微量注射到小鼠胚胎中后进行比较,并通过免疫染色和 CUT&Tag 分析γH2AX 的 DNA 裂解位点。尽管低脱靶sgRNA通常被选用于生产基因编辑动物,但γH2AX免疫荧光显示,在注射Cas9系统后15小时出现了一个相对的DSB峰,而且低脱靶sgRNA注射组峰值处的γH2AX病灶数量明显高于对照组。此外,CUT&Tag测序分析结果显示,低脱靶sgRNA注射组比对照组检测到更多的双链断裂(DSB)相关序列,且DSB相关序列的分布没有染色体特异性。DSB 相关序列的基因本体(GO)注释分析表明,这些序列主要集中在与一些重要生物过程、分子功能和细胞成分相关的基因上。总之,当使用 Cas9 系统进行基因编辑时,小鼠早期胚胎中存在许多与 sgRNA 序列无关的 DSB,而且可以在基因组中检测到与 DSB 相关的序列并对其进行定性。在使用或优化 Cas9 系统时也应考虑这些结果和方法。
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Discovery and characterization of sgRNA-sequence-independent DNA cleavage from CRISPR/Cas9 in mouse embryos

The CRISPR/Cas9 system can induce off-target effects in programmed gene editing, but there have been few reports on cleavage detection and their affection in embryo development. To study these events, sgRNAs with different off-target rates were designed and compared after micro-injected into mouse zygotes, and γH2AX was used for DNA cleavage sites analysis by immunostaining and CUT&Tag. Although the low off-target sgRNA were usually selected for production gene editing animals, γH2AX immunofluorescence indicated that there was a relative DSB peak at 15 h after Cas9 system injection, and the number of γH2AX foci at the peak was significantly higher in the low off-target sgRNA-injected group than in the control group. Further, the result of CUT&Tag sequencing analysis showed more double-strand breaks (DSBs) related sequences were detected in low off-target sgRNA-injected group than control and the distribution of DSB related sequences had no chromosome specificity. Gene Ontology (GO) annotation analysis of the DSB related sequences showed that these sequences were mainly concentrated at genes associated with some important biological processes, molecular functions, and cell components. In a conclusion, there are many sgRNA-sequence-independent DSBs in early mouse embryos when the Cas9 system is used for gene editing and the DSB related sequence could be detected and characterized in the genome. These results and method should also be considered in using or optimizing the Cas9 system.

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CiteScore
7.20
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4.30%
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567
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