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  • Turkish Journal of Veterinary and Animal Sciences
  • Volume:23 Issue:1
  • Comparative Analysis of Highly Virulent Infectious Bursal Disease Viruses Isolated in Turkey Using t...

Comparative Analysis of Highly Virulent Infectious Bursal Disease Viruses Isolated in Turkey Using the SDS-PAGE and Western Immunoblotting Techniques

Authors : Olcay TÜRE
Pages : 83-92
View : 15 | Download : 6
Publication Date : 0000-00-00
Article Type : Research Paper
Abstract :Structural protein profiles and antigenic ralatedness of the regional viruses insert ignore into journalissuearticles values(Agean:G34, G35; Marmara:G41; Central Anatolia:ETL3); isolated from the infectious bursal disease outbreaks in Turkey were examined comparatively with the serotype 1 classic insert ignore into journalissuearticles values(D78); and variant insert ignore into journalissuearticles values(E variant); strains using the SDS-PAGE insert ignore into journalissuearticles values(Sodium Dodecyl Sulphate Polyacrylamide Gel Electrophoresis); and Western immunoblotting techniques. SDS-PAGE analysis of 3 purified field insert ignore into journalissuearticles values(G34, G35, ETL3); and 1 reference insert ignore into journalissuearticles values(D78); viruses showed that local viruses had the same protein profiles with the serotype 1 reference strain. VP2insert ignore into journalissuearticles values(40K);, VP3insert ignore into journalissuearticles values(32K); and VPXinsert ignore into journalissuearticles values(48K); were the proteins identified in Coomassie blue stained gels. In this study, it was not possible to detect the other structural proteins insert ignore into journalissuearticles values(VP1 and VP4); clearly due to the cellular contaminant proteins. The polyclonal antisera to D78, E variant, G34, G35, G41 and the ETL3 strains used in Western immunoblotting tests detected mostly three protein bands, VP2, VP3 and a 52K molecular weight protein which was reported to be the precursor of VP3 in homologous and heterologous reactions. The antisera to ETL3 showed stronger reaction with VP2 of the viruses comparison to the VP3. The antisera to G35 strain reacted only with the VP3 and its precursor protein and showed no detectable reaction with the VP2 protein. In conclusion, no differences were found between the reference and the regional IBDV strains in terms of protein profiles as detected by SDS-PAGE. Western immunoblotting studies indicated that, although some differences were observed in case of ETL3 and G35 reactions, the majority of viruses tested in this study were antigenically similar.
Keywords : Highly Virulent IBDV, Proteins, Antigenic Characterization, SDS PAGE, Western Immunoblotting

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