Literature DB >> 11526146

Use of a heteroduplex mobility assay to detect differences in the fusion protein cleavage site coding sequence among Newcastle disease virus isolates.

A Berinstein1, H S Sellers, D J King, B S Seal.   

Abstract

Newcastle disease virus (NDV) is an economically important pathogen of poultry that may cause clinical disease that ranges from a mild respiratory syndrome to a virulent form with high mortality, depending on an isolate's pathotype. Infections with virulent NDV strains are required to be reported by member nations to the Office of International Epizootes (OIE). The primary determinant for virulence among NDV isolates is the presence or absence of dibasic amino acids in the fusion (F) protein cleavage activation site. Along with biological virulence determinations as the definitive tests, OIE accepts reporting of the F protein cleavage site sequence of NDV isolates as a virulence criterion. Nucleotide sequence data for many NDV isolates recently isolated from infected chickens and other avian species worldwide have been deposited in GenBank. Consequently, viral genomic information surrounding the F protein cleavage site coding sequence was used to develop a heteroduplex mobility assay (HMA) to aid in further identification of molecular markers as predictors of NDV virulence. Using common vaccine strains as a reference, we were able to distinguish virulent viruses among NDV isolates that correlated with phylogenetic analysis of the nucleotide sequence. This technique was also used to examine NDV isolates not previously characterized. We were able to distinguish vaccine-like viruses from other isolates potentially virulent for chickens. This technique will help improve international harmonization of veterinary biologics as set forth by the OIE and the Veterinary International Cooperation on Harmonization of Technical Requirements of Veterinary Medicinal Products. Ultimately, the HMA could be used for initial screening among a large number of isolates and rapid identification of potentially virulent NDV that continue to threaten commercial poultry worldwide.

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Year:  2001        PMID: 11526146      PMCID: PMC88314          DOI: 10.1128/JCM.39.9.3171-3178.2001

Source DB:  PubMed          Journal:  J Clin Microbiol        ISSN: 0095-1137            Impact factor:   5.948


  39 in total

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4.  Antigenic variation of Newcastle disease virus strains detected by monoclonal antibodies.

Authors:  P H Russell; D J Alexander
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5.  Genetic relationships determined by a DNA heteroduplex mobility assay: analysis of HIV-1 env genes.

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6.  Deduced amino acid sequences at the fusion protein cleavage site of Newcastle disease viruses showing variation in antigenicity and pathogenicity.

Authors:  M S Collins; J B Bashiruddin; D J Alexander
Journal:  Arch Virol       Date:  1993       Impact factor: 2.574

7.  An oligonucleotide probe that distinguishes isolates of low virulence from the more pathogenic strains of Newcastle disease virus.

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8.  An enzyme-linked immunosorbent assay that measures protective antibody levels to Newcastle disease virus in chickens.

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9.  Expression of factor X and its significance for the determination of paramyxovirus tropism in the chick embryo.

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10.  Simplified hepatitis C virus genotyping by heteroduplex mobility analysis.

Authors:  P A White; X Zhai; I Carter; Y Zhao; W D Rawlinson
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  6 in total

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3.  Development of a real-time reverse-transcription PCR for detection of newcastle disease virus RNA in clinical samples.

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4.  Molecular characterization and phylogenetic study of newcastle disease virus isolates from recent outbreaks in eastern Uganda.

Authors:  Maxwell O Otim; Henrik Christensen; Poul H Jørgensen; Kurt J Handberg; Magne Bisgaard
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5.  Development of a heteroduplex mobility assay to identify field isolates of porcine reproductive and respiratory syndrome virus with nucleotide sequences closely related to those of modified live-attenuated vaccines.

Authors:  K F Key; D K Guenette; K-J Yoon; P G Halbur; T E Toth; X J Meng
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6.  Reverse Genetics Assembly of Newcastle Disease Virus Genome Template Using Asis-Sal-Pac BioBrick Strategy.

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  6 in total

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