An Assessment of Diagnostic Assays and Sample Types in the Detection of an Attenuated Genotype 5 African Swine Fever Virus in European Pigs over a 3-Month Period

Author:

Havas Karyn A.ORCID,Gogin Andrey E.ORCID,Basalaeva Julia V.,Sindryakova Irina P.ORCID,Kolbasova Olga L.,Titov Ilya A.ORCID,Lyska Valentina M.,Morgunov Sergey Y.,Vlasov Mikhail E.,Sevskikh Timofey A.,Pivova Elena Y.,Kudrjashov Dmitry A.ORCID,Doolittle Kent,Zimmerman Silvia,Witbeck Wendy,Gimenez-Lirola Luis G.,Nerem Joel,Spronk Gordon D.,Zimmerman Jeffrey J.ORCID,Sereda Alexey D.

Abstract

African swine fever virus causes hemorrhagic disease in swine. Attenuated strains are reported in Africa, Europe, and Asia. Few studies on the diagnostic detection of attenuated ASF viruses are available. Two groups of pigs were inoculated with an attenuated ASFV. Group 2 was also vaccinated with an attenuated porcine reproductive and respiratory syndrome virus vaccine. Commercially available ELISA, as well as extraction and qPCR assays, were used to detect antibodies in serum and oral fluids (OF) and nucleic acid in buccal swabs, tonsillar scrapings, OF, and blood samples collected over 93 days, respectively. After 12 dpi, serum (88.9% to 90.9%) in Group 1 was significantly better for antibody detection than OF (0.7% to 68.4%). Group 1′s overall qPCR detection was highest in blood (48.7%) and OF (44.2%), with the highest detection in blood (85.2%) from 8 to 21 days post inoculation (dpi) and in OF (83.3%) from 1 to 7 dpi. Group 2′s results were not significantly different from Group 1, but detection rates were lower overall. Early detection of attenuated ASFV variants requires active surveillance in apparently healthy animals and is only reliable at the herd level. Likewise, antibody testing will be needed to prove freedom from disease.

Funder

National Pork Board

Cherkizovo LLC

Publisher

MDPI AG

Subject

Infectious Diseases,Microbiology (medical),General Immunology and Microbiology,Molecular Biology,Immunology and Allergy

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