Molecular contamination of an animal facility during and after African swine fever virus infection
Author:
Walczak Marek1ORCID, Szymankiewicz Krzesimir1ORCID, Rodriguez Fernando234ORCID, Argilaguet Jordi234ORCID, Gavrilov Boris5ORCID, Żmudzki Jacek1ORCID, Kochanowski Maciej1ORCID, Juszkiewicz Małgorzata1ORCID, Szczotka-Bochniarz Anna1ORCID
Affiliation:
1. 1 Department of Swine Diseases, National Veterinary Research Institute , Puławy , Poland 2. 2 Unitat Mixta d’Investigació IRTA-UAB en Sanitat Animal, Centre de Recerca en Sanitat Animal (CReSA), Campus de la Universitat Autònoma de Barcelona (UAB) , Bellaterra , Spain 3. 3 IRTA, Programa de Sanitat Animal, Centre de Recerca en Sanitat Animal (CReSA), Campus de la Universitat Autònoma de Barcelona (UAB) , Bellaterra , Spain 4. 4 WOAH Collaborating Centre for Emerging and Re-emerging Pig Diseases in Europe, IRTA-CReSA , Barcelona , Spain 5. 5 Biologics Development, Huvepharma , Sofia , Bulgaria
Abstract
Abstract
Introduction
The molecular contamination of an animal facility was investigated during and after an infection with highly pathogenic African swine fever virus (ASFV) among domestic pigs. The investigation evaluated the risk of indirect transmission of the disease and indicated points that may facilitate cleaning and disinfection processes.
Material and Methods
Six domestic pigs were infected oronasally with the highly pathogenic Georgia 2007 strain. Environmental samples from the floors, walls, rubber floor mats, feeders, drinkers, high-efficiency particulate-absorbing filter covers and doors were collected 7 days post infection (dpi), 7 days later and 24 h after disinfection of the facility. The samples were investigated by real-time PCR and in vitro assays to find genetic traces of ASFV and infectious virus.
Results
Typical clinical outcomes for ASF (i.e. fever, apathy, recumbency and bloody diarrhoea) were observed, and all animals died or required euthanasia before or at 9 dpi. No infectious virus was found in environmental samples at the sampling time points. Genetic traces of ASFV were found in all locations except the doors. The initial virus load was calculated using real-time PCR threshold cycle values and was the highest at the drain. A statistically significant decrease of virus load over time was found on non-porous surfaces mechanically cleaned by water (the floor and drain).
Conclusion
The gathered data confirmed different routes of virus excretion (oral and nasal, faeces and urine, and aerosol) and showed virus locations and different initial concentrations in the animal facility. Maintaining the facility with mechanical cleaning and using personal protection (gloves) and hand disinfection may efficiently minimise the risk of further virus spread. Together with the results of previously published studies, the present investigations’ failure to isolate infectious virus may suggest that if stable environmental conditions are assured, the time needed before the introduction of new herds into previously ASF-affected farm facilities could be shortened and in this way the economic losses caused by the disease outbreak mitigated.
Publisher
Walter de Gruyter GmbH
Subject
General Veterinary
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