Identification of a Novel Cleavage Site and Confirmation of the Effectiveness of NgAgo Gene Editing on RNA Targets

被引:0
|
作者
Jiayao Qu
Yali Xie
Zhaoyi Guo
Xiangting Liu
Jing Jiang
Ting Chen
Kai Li
Zheng Hu
Dixian Luo
机构
[1] Huazhong University of Science and Technology Union Shenzhen Hospital (Nanshan Hospital),Laboratory Medicine Center
[2] University of South China,Translational Medicine Institute, National & Local Joint Engineering Laboratory for High
[3] Southern Medical University,Through Molecular Diagnosis Technology, The First People’s Hospital of Chenzhou
[4] The 6th Affiliated Hospital of Shenzhen University Health Science Center,The First School of Clinical Medicine
来源
Molecular Biotechnology | 2021年 / 63卷
关键词
Argonaute; Ago; NgAgo; gDNA; RNA editing; Cleavage site;
D O I
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学科分类号
摘要
Clusters of regularly interspaced short palindromic repeats (CRISPR)/Cas systems have a powerful ability to edit DNA and RNA targets. However, the need for a specific recognition site, protospacer adjacent motif (PAM), of the CRISPR/Cas system limits its application in gene editing. Some Argonaute (Ago) proteins have endonuclease functions under the guidance of 5′ phosphorylated or hydroxylated guide DNA (gDNA). The NgAgo protein might perform RNA gene editing at 37 °C, suggesting its application in mammalian cells; however, its mechanisms are unclear. In the present study, the target of NgAgo in RNA was confirmed in vitro and in vivo. Then, an in vitro RNA cleavage system was designed and the cleavage site was verified by sequencing. Furthermore, NgAgo and gDNA were transfected into cells to cleave an intracellular target sequence. We demonstrated targeted degradation of GFP, HCV, and AKR1B10 RNAs in a gDNA-dependent manner by NgAgo both in vitro and in vivo, but no effect on DNA was observed. Sequencing demonstrated that the cleavage sites are located at the 3′ of the target RNA which is recognized by 5′ sequence of the gDNA. These results confirmed that NgAgo–gDNA cleaves RNA not DNA. We observed that the cleavage site is located at the 3′ of the target RNA, which is a new finding that has not been reported in the past.
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页码:1183 / 1191
页数:8
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