病毒蛋白酶与核小体DNA结合并切割核cGAS，从而减弱I型干扰素。

IF 5.1 1区生物学 Q1 MICROBIOLOGY

mBio Pub Date : 2025-04-09 Epub Date: 2025-02-25 DOI:10.1128/mbio.03395-24

Lei Wu, Ya Yan, Ye Yuan, Zhenchao Zhao, Weiyu Qu, Xiangyu Huang, Haiwei Wang, Pingwei Li, Xin Li

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引用次数: 0

摘要

核环GMP-AMP合成酶（cGAS）以高亲和力与核小体结合，阻止其被自身dna激活。在双链DNA的刺激下，cGAS被激活，并在其n端结构域的引导下从细胞核转运到细胞质。然而，目前尚不清楚病毒是否可以劫持cGAS易位并调节其激活。在这里，我们发现小核糖核酸病毒塞内卡谷病毒（SVV）的蛋白酶3C在病毒感染后从细胞质转运到细胞核，并与细胞核DNA结合。蛋白酶3C特异性地切割组蛋白H2A，而不影响其他组蛋白。此外，DNA结合增强了蛋白酶3C切割核cGAS的能力，导致其保留在细胞核中。这反过来又抑制了poly（dA:dT）刺激后I型干扰素（IFN-I）的诱导。这些发现揭示了一种新的机制，通过病毒蛋白酶结合核DNA，切割核cGAS和组蛋白H2A，从而错定位cGAS，促进免疫逃避。重要性：环GMP-AMP合成酶（cGAS）在细胞核中稳定表达，并被染色质紧密束缚，以防止其被自身dna激活。在刺激或感染期间，核cGAS被激活并从细胞核转运到细胞质。然而，专门针对核cGAS的病毒策略完全未被探索。在这里，我们发现Seneca Valley病毒的蛋白酶3C在病毒感染后从细胞质易位到细胞核，与核DNA结合，并特异性地切割H2A。此外，DNA与3C的结合增强了核cGAS在其n端结构域内的裂解。阻碍cGAS从细胞核到细胞质的易位导致IFN-I诱导受到抑制并导致免疫逃避。这项工作揭示了一种独特的机制，其中病毒蛋白酶结合核DNA并切割核cGAS和组蛋白H2A，导致病毒逃避cGAS介导的免疫限制。

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Viral protease binds to nucleosomal DNA and cleaves nuclear cGAS that attenuates type I interferon.

Nuclear cyclic GMP-AMP synthetase (cGAS) binds to nucleosome with high affinity to prevent its activation by self-DNA. Upon stimulation with double-stranded DNA, cGAS is activated and translocates from the nucleus to the cytoplasm, guided by its N-terminal domain. However, it remains unclear whether viruses can hijack cGAS translocation and regulate its activation. Here, we discovered that the protease 3C of picornavirus Seneca Valley virus (SVV) translocates from the cytoplasm to the nucleus upon viral infection and binds to nuclear DNA. Protease 3C specifically cleaves histone H2A while leaving other histone proteins unaffected. Additionally, DNA binding enhances the protease 3C's ability to cleave nuclear cGAS, leading to its retention in the nucleus. This, in turn, suppresses the induction of type I interferon (IFN-I) following poly(dA:dT) stimulation. These findings reveal a novel mechanism by which a viral protease binds nuclear DNA, cleaves nuclear cGAS and histone H2A, and thereby mislocalizes cGAS, facilitating immune evasion.

Importance: Cyclic GMP-AMP synthetase (cGAS) is robustly expressed in the nucleus and tightly tethered by chromatin to prevent its activation with self-DNA. During stimulation or infection, nuclear cGAS is activated and translocates from the nucleus to the cytoplasm. However, the viral strategies specifically targeting nuclear cGAS are completely unexplored. Here, we discovered that protease 3C of Seneca Valley virus translocates from the cytoplasm to the nucleus upon viral infection, binds to nuclear DNA, and specifically cleaves H2A. Furthermore, DNA binding to 3C enhances the cleavage of nuclear cGAS within its N-terminal domain. The hindrance of cGAS translocation from the nucleus to the cytoplasm results in the suppression of IFN-I induction and leads to immune evasion. This work uncovers a unique mechanism wherein a viral protease binds to nuclear DNA and cleaves nuclear cGAS and histone H2A, leading to viral evasion of cGAS-mediated immune restriction.

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来源期刊

mBio MICROBIOLOGY-

CiteScore

10.50

自引率

3.10%

发文量

762

审稿时长

1 months

期刊介绍： mBio® is ASM''s first broad-scope, online-only, open access journal. mBio offers streamlined review and publication of the best research in microbiology and allied fields.