Live vaccines predominantly control avian metapneumovirus (AMPV) infection in the poultry industry but these can persist after application and revert to virulence. Sequencing of the G gene of the dominant subtype B VCO3 vaccinal strain identified a unique nucleotide substitution (A→G, nucleotide 91) which fortuitously introduced an MseI restriction endonuclease site within the amplicon obtained from a popular AMPV diagnostic RT- nested PCR. An Msel digestion protocol was developed then validated using Italian B subtype viruses of known field virus or vaccine origin.

RAPID DIFFERENTIATION OF VACCINE AND FIELD STRAINS OF AVIAN METAPNEUMOVIRUS OF SUBTYPE B BY RESTRICTION ENZYME DIGESTION OF PCR PRODUCTS

CECCHINATO, MATTIA;
2012

Abstract

Live vaccines predominantly control avian metapneumovirus (AMPV) infection in the poultry industry but these can persist after application and revert to virulence. Sequencing of the G gene of the dominant subtype B VCO3 vaccinal strain identified a unique nucleotide substitution (A→G, nucleotide 91) which fortuitously introduced an MseI restriction endonuclease site within the amplicon obtained from a popular AMPV diagnostic RT- nested PCR. An Msel digestion protocol was developed then validated using Italian B subtype viruses of known field virus or vaccine origin.
2012
VII. International Symposium on Avian Corona and Pneumovirus and Complicating Pathogens
9783980590792
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/11577/2534664
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