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Cryo-EM structure of the vaccinia virus entry fusion complex reveals a multicomponent fusion machinery

Chang Sheng‐Huei Lin, Ching-An Li, Chun-Hsiung Wang, Chi-Fei Kao, Hsiao-Jung Chiu, Min-Chi Yeh, Hua-De Gao, Meng-Chiao Ho, Hsien-Ming Lee, W. C. Chang

2026Science Advances6 citationsDOIOpen Access PDF

Abstract

Membrane fusion is essential for viral entry. Unlike class I-III fusion proteins, vaccinia virus (VACV) uses a multicomponent entry fusion complex (EFC). Using cryo-electron microscopy, we determined the full-length structure of the VACV EFC at near-atomic resolution, revealing a 15-protein asymmetric assembly organized into three layers. The central A16/G9/J5 heterotrimer forms the fusion core, stabilized by conserved PXXCW and Delta motifs, and anchors two A28/H2 adaptor dimers linked to peripheral G3/L5/A21/O3 scaffolds. Structural and evolutionary analyses identify a conserved N-terminal domain in A16 containing a myristoyl-binding pocket and a phenylalanine-rich region that stabilizes the trimer and may regulate lipid engagement. An additional component, F9, binds peripherally to J5, A21, and H2 through Delta-like motifs, reinforcing the prefusion architecture. Together, these results define the VACV EFC as a unique multiprotein fusion machinery and provide a structural framework for understanding the mechanism of poxvirus entry and membrane fusion.

Topics & Concepts

Lipid bilayer fusionFusion mechanismFusionVacciniaTrimerCell biologyViral entryViral envelopeVirusBiologyComputational biologyFusion proteinBiophysicsChemistryProtein structureVirologySignal transducing adaptor proteinOrthopoxvirusPlasma protein bindingPoxviridaeCell fusionViral membraneMechanism (biology)Protein domainViral proteinDomain (mathematical analysis)Multiprotein complexVirus classificationPoxvirus research and outbreaksInfluenza Virus Research StudiesBacteriophages and microbial interactions
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