Lin Ren-Jye, Lin Li-Hsiung, Chen Zih-Ping, Liu Bing-Cheng, Ko Pin-Chen, Liao Ching-Len
National Mosquito-Borne Diseases Control Research Center, National Health Research Institute, Taipei, Taiwan.
National Institute of Infectious Diseases and Vaccinology, National Health Research Institutes, Miaoli, Taiwan.
J Biomed Sci. 2025 Feb 20;32(1):27. doi: 10.1186/s12929-025-01122-0.
The zinc finger protein 36-like (ZFP36L) family is a CCCH-type group consisting of RNA-binding proteins, i.e., ZFP36L1 and ZFP36L2, which regulate cellular mRNA through the RNA decay pathway. ZFP36L1 combats flavivirus infections through the 5'-3' XRN1 and 3'-5' RNA exosome decay pathways. The present study clarified the role of human ZFP36L2 in the defense response of the host against flavivirus infection.
Cell lines with overexpression or knockdown of ZFP36L2 were established using lentiviral vectors carrying genes for overexpression and short-hairpin RNA targeting specific genes, respectively. A plaque assay was employed to determine the viral titer. Immunofluorescence and real-time quantitative polymerase chain reaction were used to measure the viral RNA levels. The in vitro-transcribed RNA transcript derived from a replication-dead Japanese encephalitis virus (JEV) replicon containing the renilla luciferase reporter gene (J-R2A-NS5mt) was used to assess the stability of the flavivirus RNA. An RNA immunoprecipitation assay was used to detect the protein-RNA binding ability. Confocal microscopic images were captured to analyze protein colocalization.
ZFP36L2 served as an innate host defender against JEV and dengue virus. ZFP36L2 inhibited flavivirus infection solely through the 5'-3' XRN1 RNA decay pathway, whereas ZFP36L1 inhibited JEV infection via the 5'-3' XRN1 and 3'-5' RNA exosome RNA decay pathways. The direct binding between viral RNA and ZFP36L2 via its CCCH-type zinc finger motifs facilitated the degradation of flavivirus RNA mediated by 5'-3' XRN1. Furthermore, ZFP36L2 was localized in processing bodies (PBs), which participate in the 5'-3' XRN1-mediated RNA decay pathway. Nonetheless, the disruption of PBs did not affect the antiviral activity of ZFP36L2, suggesting that its localization is not essential for the function of the protein. Interestingly, the colocalization of ZFP36L2 and XRN1 with viral RNA and NS3 revealed that the antiviral activity of ZFP36L2 occurred within the replication complexes (RCs).
In summary, ZFP36L2 bound to and degraded viral RNA through the XRN1-mediated RNA decay pathway in the RCs, thereby inhibiting flavivirus replication. These findings provide valuable insights into the diverse antiviral mechanisms of the ZFP36-like family of proteins in the innate immune response against flavivirus infection.
锌指蛋白36样(ZFP36L)家族是一个由RNA结合蛋白组成的CCCH型家族,即ZFP36L1和ZFP36L2,它们通过RNA降解途径调节细胞mRNA。ZFP36L1通过5'-3' XRN1和3'-5' RNA外切体降解途径对抗黄病毒感染。本研究阐明了人ZFP36L2在宿主抗黄病毒感染防御反应中的作用。
分别使用携带过表达基因和靶向特定基因的短发夹RNA的慢病毒载体建立ZFP36L2过表达或敲低的细胞系。采用蚀斑试验测定病毒滴度。免疫荧光和实时定量聚合酶链反应用于测量病毒RNA水平。使用来自含有海肾荧光素酶报告基因的复制缺陷型日本脑炎病毒(JEV)复制子(J-R2A-NS5mt)的体外转录RNA转录本评估黄病毒RNA的稳定性。采用RNA免疫沉淀试验检测蛋白质-RNA结合能力。拍摄共聚焦显微镜图像以分析蛋白质共定位。
ZFP36L2作为宿主抵御JEV和登革病毒的天然防御因子。ZFP36L2仅通过5'-3' XRN1 RNA降解途径抑制黄病毒感染,而ZFP36L1通过5'-3' XRN1和3'-5' RNA外切体RNA降解途径抑制JEV感染。病毒RNA与ZFP36L2通过其CCCH型锌指基序直接结合,促进了5'-3' XRN1介导的黄病毒RNA降解。此外,ZFP36L2定位于加工小体(PBs),其参与5'-3' XRN1介导的RNA降解途径。然而,PBs的破坏并不影响ZFP36L2的抗病毒活性,表明其定位对该蛋白的功能并非必不可少。有趣的是,ZFP36L2和XRN1与病毒RNA和NS3的共定位表明,ZFP36L2的抗病毒活性发生在复制复合物(RCs)内。
总之,ZFP36L2通过RCs中XRN1介导的RNA降解途径与病毒RNA结合并使其降解,从而抑制黄病毒复制。这些发现为ZFP36样蛋白家族在抗黄病毒感染的先天免疫反应中的多种抗病毒机制提供了有价值的见解。
Zotero 插件
