Genre
- Journal Article
The baculovirus expression vector system was used to examine the expression of the full-length infectious bursal disease virus (IBDV) segment A cDNA, which encodes the structural proteins in a polyprotein precursor that is autocatalytically cleaved to VPX, VP3, and VP4. No VP2 was observed in lysates of recombinant baculovirus infected cells indicating the lack of processing of VPX to VP2 in this system. Virus-like particles (VLP) were purified from the infected insect cells, and on negative staining electron microscopy, looked very similar to authentic IBDV particles in shape and size, suggesting that processing of VPX to VP2 is not necessary for capsid assembly.
Department of Pathology and Microbiology, Atlantic Veterinary College, University of Prince Edward Island, Charlottetown. kibenge@upei.ca
CANADA
LR: 20061115; PUBM: Print; JID: 8607793; 0 (DNA, Complementary); 0 (Protein Precursors); 0 (Viral Proteins); ppublish
Source type: Electronic(1)
Language
- English
Subjects
- animals
- Genetic Vectors
- DNA, Complementary/genetics
- Infectious bursal disease virus/genetics
- Virus Assembly
- Gene Expression Regulation, Viral
- Protein Precursors/genetics
- Poultry Diseases/genetics/virology
- Viral Proteins/genetics
- Baculoviridae/genetics
- Chickens/virology