Department of Microbiology and Immunology, Indiana University School of Medicine Indianapolis, Indianapolis, Indiana, USA.
Department of Infectious Diseases, Huashan Hospital, Fudan Universitygrid.8547.e, Shanghai, China.
J Virol. 2021 Sep 9;95(19):e0044421. doi: 10.1128/JVI.00444-21.
DDX17 is a member of the DEAD-box helicase family proteins involved in cellular RNA folding, splicing, and translation. It has been reported that DDX17 serves as a cofactor of host zinc finger antiviral protein (ZAP)-mediated retroviral RNA degradation and exerts direct antiviral function against Raft Valley fever virus through binding to specific stem-loop structures of viral RNA. Intriguingly, we have previously shown that ZAP inhibits hepatitis B virus (HBV) replication through promoting viral RNA decay, and the ZAP-responsive element (ZRE) of HBV pregenomic RNA (pgRNA) contains a stem-loop structure, specifically epsilon, which serves as the packaging signal for pgRNA encapsidation. In this study, we demonstrated that the endogenous DDX17 is constitutively expressed in human hepatocyte-derived cells but dispensable for ZAP-mediated HBV RNA degradation. However, DDX17 was found to inhibit HBV replication primarily by reducing the level of cytoplasmic encapsidated pgRNA in a helicase-dependent manner. Immunofluorescence assay revealed that DDX17 could gain access to cytoplasm from nucleus in the presence of HBV RNA. In addition, RNA immunoprecipitation and electrophoretic mobility shift assays demonstrated that the enzymatically active DDX17 competes with HBV polymerase to bind to pgRNA at the 5' epsilon motif. In summary, our study suggests that DDX17 serves as an intrinsic host restriction factor against HBV through interfering with pgRNA encapsidation. Hepatitis B virus (HBV) chronic infection, a long-studied but yet incurable disease, remains a major public health concern worldwide. Given that HBV replication cycle highly depends on host factors, deepening our understanding of the host-virus interaction is thus of great significance in the journey of finding a cure. In eukaryotic cells, RNA helicases of the DEAD box family are highly conserved enzymes involved in diverse processes of cellular RNA metabolism. Emerging data have shown that DDX17, a typical member of the DEAD box family, functions as an antiviral factor through interacting with viral RNA. In this study, we, for the first time, demonstrate that DDX17 inhibits HBV through blocking the formation of viral replication complex, which not only broadens the antiviral spectrum of DDX17 but also provides new insight into the molecular mechanism of DDX17-mediated virus-host interaction.
DDX17 是 DEAD-box 解旋酶家族蛋白的成员,参与细胞 RNA 折叠、剪接和翻译。有报道称,DDX17 作为宿主锌指抗病毒蛋白 (ZAP) 介导的逆转录病毒 RNA 降解的辅助因子发挥作用,并通过与病毒 RNA 的特定茎环结构结合发挥直接抗病毒作用对抗裂谷热病毒。有趣的是,我们之前已经表明,ZAP 通过促进病毒 RNA 降解来抑制乙型肝炎病毒 (HBV) 的复制,而 HBV 前基因组 RNA (pgRNA) 的 ZAP 反应元件 (ZRE) 包含一个茎环结构,特别是 ε,它作为 pgRNA 包裹的包装信号。在这项研究中,我们证明内源性 DDX17 在人肝细胞源性细胞中持续表达,但对 ZAP 介导的 HBV RNA 降解不是必需的。然而,发现 DDX17 主要通过以解旋酶依赖的方式降低细胞质中包裹的 pgRNA 水平来抑制 HBV 复制。免疫荧光检测显示,在 HBV RNA 的存在下,DDX17 可以从核内进入细胞质。此外,RNA 免疫沉淀和电泳迁移率变动分析表明,具有酶活性的 DDX17 与 HBV 聚合酶竞争结合 pgRNA 的 5'ε 基序。总之,我们的研究表明,DDX17 通过干扰 pgRNA 包裹作为一种内在的宿主限制因子来抑制 HBV。乙型肝炎病毒 (HBV) 慢性感染是一种长期研究但仍无法治愈的疾病,仍然是全球主要的公共卫生关注点。鉴于 HBV 的复制周期高度依赖于宿主因素,因此深入了解宿主-病毒相互作用对于寻找治疗方法具有重要意义。在真核细胞中,DEAD 盒家族的 RNA 解旋酶是高度保守的酶,参与细胞 RNA 代谢的多种过程。新出现的数据表明,DDX17,一种典型的 DEAD 盒家族成员,通过与病毒 RNA 相互作用发挥抗病毒作用。在这项研究中,我们首次证明 DDX17 通过阻断病毒复制复合物的形成来抑制 HBV,这不仅拓宽了 DDX17 的抗病毒谱,而且为 DDX17 介导的病毒-宿主相互作用的分子机制提供了新的见解。