Infectious bursal disease viruses: molecular differentiation of antigenic subtypes among serotype 1 viruses

Published nucleotide sequence data for IBDV variant viruses (A and 1048E) and classic viruses (STC, 52-70, PBG98, Cu-1, and 002-73) were used to identify restriction enzyme sites that could potentially be used to differentiate these strains of IBDV. To test this hypothesis, the genomes of IBDV strai...

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Bibliographic Details
Published inAvian diseases Vol. 38; no. 3; p. 531
Main Authors Jackwood, D.J. (Ohio State University, Wooster, OH.), Jackwood, R.J
Format Journal Article
LanguageEnglish
Published United States 01.07.1994
Subjects
AMPLIFICATION CHAINE POLYMERASE
Animals
Antigens, Viral - classification
Antigens, Viral - genetics
Birnaviridae Infections - diagnosis
Birnaviridae Infections - veterinary
Birnaviridae Infections - virology
Capsid - genetics
Capsid - immunology
Capsid Proteins
Chickens
DIAGNOSTIC
DIAGNOSTICO
DIFERENCIAS BIOLOGICAS
DIFFERENCE BIOLOGIQUE
DNA, Viral - genetics
ENFERMEDAD DE GUMBORO
Genes, Viral
Genetic Variation
Infectious bursal disease virus - classification
Infectious bursal disease virus - genetics
Infectious bursal disease virus - immunology
MALADIE DE GUMBORO
NUCLEASAS
NUCLEASE
Polymerase Chain Reaction
Poultry Diseases - diagnosis
Poultry Diseases - prevention & control
Poultry Diseases - virology
REACCION DE CADENAS DE POLIMERASA
Restriction Mapping
SECUENCIA NUCLEICA
SEQUENCE NUCLEIQUE
Serotyping
TRANSCRIPTASA INVERSA
TRANSCRIPTASE INVERSE
Turkeys
Viral Vaccines - isolation & purification
Virulence - genetics
Virulence - immunology
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Summary:Published nucleotide sequence data for IBDV variant viruses (A and 1048E) and classic viruses (STC, 52-70, PBG98, Cu-1, and 002-73) were used to identify restriction enzyme sites that could potentially be used to differentiate these strains of IBDV. To test this hypothesis, the genomes of IBDV strains STC, MD, NC, and OH were converted to cDNA using reverse transcriptase (RT) and then amplified using the polymerase chain reaction (PCR). The PCR primers were selected from relatively conserved sequence regions in the VP2 gene, and they were used to amplify a 394-base-pair fragment. The restriction enzymes (RE) DraI, EcoRII, SacI, Sau3AI, StyI, and TaqI were tested for their ability to digest the RT/PCR products. The STC classic virus was SacI-, StyI-, and EcoRII-positive and DraI-, Sau3AI-, and TaqI-negative. The MD, NC, and OH viruses were DraI-, Sau3AI-, and TaqI-positive and SacI-, StyI-, and EcoRII-negative. The classic STC strain could be differentiated from the variant MD strain using the RT/PCR-RE assay. Based on these results and the presence or absence of other restriction sites that were predicted by published nucleotide sequence data, the RT/PCR-RE assay has the potential to differentiate IBDV isolates MD, A, and 1048E. Published nucleotide sequence data and the RT/PCR-RE results obtained using STC and MD indicated that variant viruses MD, A, and 1048E could be differentiated from classic viruses STC, 52-70, PBG98, Cu-1, 002-73, and NC
Bibliography:9533450
L73
ISSN:0005-2086
1938-4351
DOI:10.2307/1592075