The collateral activity of RfxCas13d can induce lethality in a RfxCas13d knock-in mouse model

Author:

Li YunfeiORCID,Xu Junjie,Guo Xuefei,Li Zhiwei,Cao Lili,Liu Shengde,Guo Ying,Wang Guodong,Luo Yujie,Zhang Zeming,Wei Xuemei,Zhao Yingchi,Liu Tongtong,Wang Xiao,Xia Huawei,Kuang Ming,Guo Qirui,Li Junhong,Chen Luoying,Wang Yibing,Li Qi,Wang Fengchao,Liu Qinghua,You Fuping

Abstract

Abstract Background The CRISPR-Cas13 system is an RNA-guided RNA-targeting system and has been widely used in transcriptome engineering with potentially important clinical applications. However, it is still controversial whether Cas13 exhibits collateral activity in mammalian cells. Results Here, we find that knocking down gene expression using RfxCas13d in the adult brain neurons caused death of mice, which may result from the collateral activity of RfxCas13d rather than the loss of target gene function or off-target effects. Mechanistically, we show that RfxCas13d exhibits collateral activity in mammalian cells, which is positively correlated with the abundance of target RNA. The collateral activity of RfxCas13d could cleave 28s rRNA into two fragments, leading to translation attenuation and activation of the ZAKα-JNK/p38-immediate early gene pathway. Conclusions These findings provide new mechanistic insights into the collateral activity of RfxCas13d in mammalian cells and warn that the biosafety of the CRISPR-Cas13 system needs further evaluation before application to clinical treatments.

Funder

National Key Research and Development Program of China

Publisher

Springer Science and Business Media LLC

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