Database of articles cited by EMDB/PDB/SASBDB data

Keywords
Structure methods	All X-ray diffraction NMR electron microscopy small angle scattering neutron diffraction fiber diffraction powder diffraction infrared spectroscopy EPR fluorescence transfer theoretical model Hybrid
Author
Journal
IF	>30 >20 >10 >5 all

Title	Bluetongue virus capsid protein VP5 perforates membranes at low endosomal pH during viral entry.
Journal, issue, pages	Nat Microbiol, Vol. 6, Issue 11, Page 1424-1432, Year 2021
Publish date	Oct 26, 2021
Authors	Xian Xia / Weining Wu / Yanxiang Cui / Polly Roy / Z Hong Zhou /
PubMed Abstract	Bluetongue virus (BTV) is a non-enveloped virus and causes substantial morbidity and mortality in ruminants such as sheep. Fashioning a receptor-binding protein (VP2) and a membrane penetration ...Bluetongue virus (BTV) is a non-enveloped virus and causes substantial morbidity and mortality in ruminants such as sheep. Fashioning a receptor-binding protein (VP2) and a membrane penetration protein (VP5) on the surface, BTV releases its genome-containing core (VP3 and VP7) into the host cell cytosol after perforation of the endosomal membrane. Unlike enveloped ones, the entry mechanisms of non-enveloped viruses into host cells remain poorly understood. Here we applied single-particle cryo-electron microscopy, cryo-electron tomography and structure-guided functional assays to characterize intermediate states of BTV cell entry in endosomes. Four structures of BTV at the resolution range of 3.4-3.9 Å show the different stages of structural rearrangement of capsid proteins on exposure to low pH, including conformational changes of VP5, stepwise detachment of VP2 and a small shift of VP7. In detail, sensing of the low-pH condition by the VP5 anchor domain triggers three major VP5 actions: projecting the hidden dagger domain, converting a surface loop to a protonated β-hairpin that anchors VP5 to the core and stepwise refolding of the unfurling domains into a six-helix stalk. Cryo-electron tomography structures of BTV interacting with liposomes show a length decrease of the VP5 stalk from 19.5 to 15.5 nm after its insertion into the membrane. Our structures, functional assays and structure-guided mutagenesis experiments combined indicate that this stalk, along with dagger domain and the WHXL motif, creates a single pore through the endosomal membrane that enables the viral core to enter the cytosol. Our study unveils the detailed mechanisms of BTV membrane penetration and showcases general methods to study cell entry of other non-enveloped viruses.
External links	Nat Microbiol / PubMed:34702979 / PubMed Central
Methods	EM (single particle)
Resolution	3.4 - 3.9 Å
Structure data	24684 7rtn EMDB-24684, PDB-7rtn: Cryo-EM structure of bluetongue virus capsid protein VP5 at low endosomal pH Method: EM (single particle) / Resolution: 3.4 Å 24685 7rto EMDB-24685, PDB-7rto: Cryo-EM structure of bluetongue virus capsid protein VP5 at low endosomal pH intermediate state 2 Method: EM (single particle) / Resolution: 3.8 Å EMDB-24686: Cryo-EM structure of bluetongue virus capsid protein VP5 at low endosomal pH intermediate state 1 Method: EM (single particle) / Resolution: 3.9 Å EMDB-24687: Cryo-EM structure of bluetongue virus capsid protein at low endosomal pH intermediate state 3 Method: EM (single particle) / Resolution: 3.6 Å
Source	bluetongue virus (serotype 1 / isolate south africa)
Keywords	VIRAL PROTEIN / Bluetongue virus / capsid / membrane penetration / VP5