State Key Laboratory of Crop Stress Biology for Arid Areas, Key Laboratory of Northwest Loess Plateau Crop Pest Management of Ministry of Agriculture, College of Plant Protection, Northwest A&F University, Yangling, China.
Key Laboratory of Integrated Crop Pest Management of Shandong Province, College of Plant Health and Medicine, Qingdao Agricultural University, Qingdao, China.
J Virol. 2020 Sep 15;94(19). doi: 10.1128/JVI.01105-20.
Autographa californica multiple nucleopolyhedrovirus (AcMNPV) GP64 is a class III viral fusion protein that mediates low-pH-triggered membrane fusion during virus entry. Although the structure of GP64 in a postfusion conformation has been solved, its prefusion structure and the mechanism of how the protein refolds to execute fusion are unknown. In its postfusion structure, GP64 is composed of five domains (domains I to V). Domain IV (amino acids [aa] 374 to 407) contains two loops (loop 1 and loop 2) that form a hydrophobic pocket at the membrane-distal end of the molecule. To determine the roles of domain IV, we used alanine-scanning mutagenesis to replace each of the individual residues and the contact-forming residues within domain IV and evaluate their contributions to GP64-mediated membrane fusion and virus infection. In many cases, replacement of a single amino acid had no significant impact on GP64. However, replacement of R392 or disruption of the N381-N385, N384-Y388, N385-W393, or K389-W393 contact resulted in poor cell surface expression and fusion loss of the modified GP64, whereas replacement of E390 or G391 or disruption of the N381-K389, N381-Q401, or N381-I403 contact reduced the cell surface expression level of the constructs and the ability of GP64 to mediate fusion pore expansion. In contrast, replacement of N407 or disruption of contact D404-S406 appeared to restrict fusion pore expansion without affecting expression. Combined with the finding that these constructs remain in the prefusion conformation or have a dramatically less efficient transition from the prefusion to the postfusion state under acidic conditions, we proposed that domain IV is necessary for refolding of GP64 during membrane fusion. Baculovirus GP64 is grouped with rhabdovirus G, herpesvirus gB, and thogotovirus glycoproteins as a class III viral fusion protein. In their postfusion structures, these proteins contain five domains (domains I to V). Distinct from domain IV of rhabdovirus G and herpesvirus gB proteins, which is composed of β-sheets, domain IV of GP64 is a loop region; the same domain in thogotovirus glycoproteins has not been solved. In addition, domain IV is proximal to domain I (fusion domain) in prefusion structures of vesicular stomatitis virus (VSV) G and human cytomegalovirus (HCMV) gB but resides at the domain I-distal end of the molecule in a postfusion conformation. In this study, we identified that highly conserved residues and contacts within domain IV of AcMNPV GP64 are necessary for low-pH-triggered conformational change and fusion pore expansion. Our results highlight the roles of domain IV of class III viral fusion proteins in refolding during membrane fusion.
美洲棉铃象鼻虫多角体病毒(AcMNPV)GP64 是一种 III 类病毒融合蛋白,它在病毒进入时介导低 pH 值触发的膜融合。尽管 GP64 在融合后构象中的结构已被解决,但它在融合前构象中的结构以及该蛋白如何重新折叠以执行融合的机制尚不清楚。在其融合后构象中,GP64 由五个结构域(结构域 I 至 V)组成。结构域 IV(氨基酸 [aa]374 至 407)包含两个环(环 1 和环 2),在分子的膜远端形成一个疏水性口袋。为了确定结构域 IV 的作用,我们使用丙氨酸扫描诱变来取代结构域 IV 内的每个单独残基和形成接触的残基,并评估它们对 GP64 介导的膜融合和病毒感染的贡献。在许多情况下,单个氨基酸的替换对 GP64 没有显著影响。然而,替换 R392 或破坏 N381-N385、N384-Y388、N385-W393 或 K389-W393 接触导致修饰的 GP64 的细胞表面表达和融合丧失,而替换 E390 或 G391 或破坏 N381-K389、N381-Q401 或 N381-I403 接触会降低构建体的细胞表面表达水平和 GP64 介导融合孔扩展的能力。相比之下,替换 N407 或破坏接触 D404-S406 似乎限制了融合孔的扩展,而不影响表达。结合这些构建体在酸性条件下仍保持融合前构象或从融合前状态向融合后状态的转换效率显著降低的发现,我们提出结构域 IV 是 GP64 在膜融合过程中重新折叠所必需的。杆状病毒 GP64 与弹状病毒 G、疱疹病毒 gB 和 Thogotovirus 糖蛋白一起被归类为 III 类病毒融合蛋白。在它们的融合后构象中,这些蛋白包含五个结构域(结构域 I 至 V)。与弹状病毒 G 和疱疹病毒 gB 蛋白的结构域 IV 不同,结构域 IV 由β-折叠组成,GP64 的结构域 IV 是一个环区;同一种蛋白在 Thogotovirus 糖蛋白中的结构域尚未解决。此外,在融合前构象中,结构域 IV 靠近水疱性口炎病毒(VSV)G 和人巨细胞病毒(HCMV)gB 的结构域 I(融合结构域),但在融合后构象中位于分子的结构域 I 远端。在这项研究中,我们确定了美洲棉铃象鼻虫多角体病毒 GP64 结构域 IV 内高度保守的残基和接触对于低 pH 值触发的构象变化和融合孔扩展是必要的。我们的结果强调了 III 类病毒融合蛋白结构域 IV 在膜融合过程中重折叠中的作用。
