Essential role of the unordered VP2 n-terminal domain of the parvovirus MVM capsid in nuclear assembly and endosomal enlargement of the virion fivefold channel for cell entry

Abstract The unordered N-termini of parvovirus capsid proteins (Nt) are translocated through a channel at the icosahedral five-fold axis to serve for virus traffick. Heterologous peptides were genetically inserted at the Nt of MVM to study their functional tolerance to manipulations. Insertion of a...

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Bibliographic Details
Published in:Virology (New York, N.Y.) N.Y.), 2012-10, Vol.432 (1), p.45-56
Main Authors: Sánchez-Martínez, Cristina, Grueso, Esther, Carroll, Miles, Rommelaere, Jean, Almendral, José M
Format: Article
Language:English
Subjects:
60 APPLIED LIFE SCIENCES
Animals
ANTIBODIES
Assembly
Capsid cleavage
Capsid Proteins - genetics
Capsid Proteins - metabolism
Cell entry
Cell Line
Cell Nucleus - virology
CLEAVAGE
Endosomes - virology
Infectious Disease
INFECTIVITY
Mice
Minute Virus of Mice - physiology
Models, Biological
Parvovirus
Peptide insertion
PEPTIDES
Protein Structure, Tertiary
Virus Assembly
Virus Internalization
Virus traffick
VIRUSES
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Summary:Abstract The unordered N-termini of parvovirus capsid proteins (Nt) are translocated through a channel at the icosahedral five-fold axis to serve for virus traffick. Heterologous peptides were genetically inserted at the Nt of MVM to study their functional tolerance to manipulations. Insertion of a 5T4-single-chain antibody at VP2-Nt (2Nt) yielded chimeric capsid subunits failing to enter the nucleus. The VEGFR2-binding peptide (V1) inserted at both 2Nt and VP1-Nt efficiently assembled in virions, but V1 disrupted VP1 and VP2 entry functions. The VP2 defect correlated with restricted externalization of V1-2Nt out of the coat. The specific infectivity of MVM and wtVP-pseudotyped mosaic MVM-V1 virions, upon heating and/or partial 2Nt cleavage, demonstrated that some 2Nt domains become intracellularly translocated out of the virus shell and cleaved to initiate entry. The V1 insertion defines a VP2-driven endosomal enlargement of the channel as an essential structural rearrangement performed by the MVM virion to infect.
ISSN:0042-6822
1096-0341
DOI:10.1016/j.virol.2012.05.025