4.4 Article

The structure of avian polyomavirus reveals variably sized capsids, non-conserved inter-capsomere interactions, and a possible location of the minor capsid protein VP4

Journal

VIROLOGY
Volume 411, Issue 1, Pages 142-152

Publisher

ACADEMIC PRESS INC ELSEVIER SCIENCE
DOI: 10.1016/j.virol.2010.12.005

Keywords

Arginine; Capsomere connections; Cryo-electron microscopy; Homology model; Human JC polyomavirus; Simian virus 40; Size-exclusion chromatography; Three-dimensional reconstruction; Virus assembly; Virus structure

Categories

Funding

  1. Brigham Young University
  2. BYU Cancer Research Center
  3. Deutsche Forschungsgesellschaft [JO 369/3-2]
  4. Ruth L. Kirschstein National Research Service Award [(F32) 1F32NS070687]
  5. National Institutes of Health [R37-GM033050]
  6. University of California [05-10505]
  7. NIH, National Cancer Institute [AI066287-01A1, CA093373-06S1]
  8. NIH [R01NS043097, P41 RR-01081]

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Avian polyomavirus (APV) causes a fatal, multi-organ disease among several bird species. Using cryogenic electron microscopy and other biochemical techniques, we investigated the structure of APV and compared it to that of mammalian polyomaviruses, particularly JC polyomavirus and simian virus 40. The structure of the pentameric major capsid protein (VP1) is mostly conserved: however, APV VP1 has a unique, truncated C-terminus that eliminates an intercapsomere-connecting beta-hairpin observed in other polyomaviruses. We postulate that the terminal beta-hairpin locks other polyomavirus capsids in a stable conformation and that absence of the hairpin leads to the observed capsid size variation in APV. Plug-like density features were observed at the base of the VP1 pentamers, consistent with the known location of minor capsid proteins VP2 and VP3. However, the plug density is more prominent in APV and may include VP4, a minor capsid protein unique to bird polyomaviruses. (C) 2010 Elsevier Inc. All rights reserved.

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