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XB-ART-23225
Proc Natl Acad Sci U S A 1992 Nov 01;8921:10046-50.
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Hepatitis B virus capsid particles are assembled from core-protein dimer precursors.

Zhou S , Standring DN .


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Our studies on the assembly of hepatitis B virus capsids or core particles in Xenopus oocytes have demonstrated that unassembled p21.5 core proteins ("free p21.5") provide a pool of low-molecular-mass precursors for core-particle assembly. Here we have characterized this material. Free p21.5 sedimented through gradients of 3-25% sucrose (wt/vol) as a single protein species of approximately 40 kDa, corresponding to a p21.5 dimer. On nonreducing SDS/polyacrylamide gels, free p21.5 migrated as disulfide-linked p21.5 dimeric species of 35 and 37 kDa. Truncated core proteins lacking most or all of the 36-amino acid protamine region at the p21.5 carboxyl terminus were also found to behave as disulfide-linked dimers with appropriately reduced molecular masses. Our experiments failed to reveal monomeric core proteins or stable intermediates between dimers and capsids along the assembly pathway. We conclude that hepatitis B virus core particles are most likely assembled by aggregating 90 (or possibly 180) disulfide-linked p21.5 dimers. We discuss similarities between the assembly of hepatitis B virus capsids and simple T = 3 plant virus and bacteriophage structures.

???displayArticle.pubmedLink??? 1438193
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Species referenced: Xenopus
Genes referenced: cdkn1a nsg1

References [+] :
Beckett, Ribonucleoprotein complexes of R17 coat protein and a translational operator analog. 1988, Pubmed