An anti-CRISPR protein disables type V Cas12a by acetylation

被引:0
|
作者
Liyong Dong
Xiaoyu Guan
Ningning Li
Fan Zhang
Yuwei Zhu
Kuan Ren
Ling Yu
Fengxia Zhou
Zhifu Han
Ning Gao
Zhiwei Huang
机构
[1] Harbin Institute of Technology,HIT Center for Life Sciences, School of Life Science and Technology
[2] Peking University,State Key Laboratory of Membrane Biology, Peking
[3] Tsinghua University,Tsinghua Center for Life Sciences, School of Life Sciences
来源
Nature Structural & Molecular Biology | 2019年 / 26卷
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摘要
Phages use anti-CRISPR proteins to deactivate the CRISPR–Cas system. The mechanisms for the inhibition of type I and type II systems by anti-CRISPRs have been elucidated. However, it has remained unknown how the type V CRISPR–Cas12a (Cpf1) system is inhibited by anti-CRISPRs. Here we identify the anti-CRISPR protein AcrVA5 and report the mechanisms by which it inhibits CRISPR–Cas12a. Our structural and biochemical data show that AcrVA5 functions as an acetyltransferase to modify Moraxella bovoculi (Mb) Cas12a at Lys635, a residue that is required for recognition of the protospacer-adjacent motif. The AcrVA5-mediated modification of MbCas12a results in complete loss of double-stranded DNA (dsDNA)-cleavage activity. In contrast, the Lys635Arg mutation renders MbCas12a completely insensitive to inhibition by AcrVA5. A cryo-EM structure of the AcrVA5-acetylated MbCas12a reveals that Lys635 acetylation provides sufficient steric hindrance to prevent dsDNA substrates from binding to the Cas protein. Our study reveals an unprecedented mechanism of CRISPR–Cas inhibition and suggests an evolutionary arms race between phages and bacteria.
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页码:308 / 314
页数:6
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