The Scrapie Prevalence in a Goat Herd Is Underestimated by Using a Rapid Diagnostic Test

Timm Konold; John Spiropoulos; Jemma Thorne; Laura Phelan; Louise Fothergill; Brenda Rajanayagam; Tobias Floyd; Beatriz Vidana; Judith Charnley; Nadya Coates; Marion Simmons

doi:10.3389/fbioe.2020.00164

The Scrapie Prevalence in a Goat Herd Is Underestimated by Using a Rapid Diagnostic Test

Front Bioeng Biotechnol. 2020 Mar 12:8:164. doi: 10.3389/fbioe.2020.00164. eCollection 2020.

Authors

Affiliations

¹ Pathology Department, Animal and Plant Health Agency Weybridge, Addlestone, United Kingdom.
² Central Sequencing Unit, Animal and Plant Health Agency Weybridge, Addlestone, United Kingdom.
³ Department of Epidemiological Sciences, Animal and Plant Health Agency Weybridge, Addlestone, United Kingdom.
⁴ Animal and Plant Health England Field Delivery, Skipton, United Kingdom.
⁵ TSE/BVDV Testing Laboratory, Eurofins Forensic Services, Risley, United Kingdom.

Abstract

Current European surveillance regulations for scrapie, a naturally occurring transmissible spongiform encephalopathy (TSE) or prion disease in sheep and goats, require testing of fallen stock or healthy slaughter animals, and outline measures in the case of confirmation of disease. An outbreak of classical scrapie in a herd with 2500 goats led to the culling of the whole herd, providing the opportunity to examine a subset of goats, take samples, and examine them for the presence of disease-associated prion protein (PrP^Sc) to provide further information on scrapie test sensitivity, pathology, and association with prion protein genotype. Goats were examined clinically prior to cull, and the brains examined post mortem by Bio-Rad ELISA, a rapid screening test used for active surveillance in sheep and goats, and two confirmatory tests, Western blot and immunohistochemistry. Furthermore, up to 10 lymphoid tissues were examined by immunohistochemistry. Of 151 goats examined, three (2.0%) tested positive for scrapie by ELISA on brain, confirmed by confirmatory tests, and a further five (3.3%) were negative by ELISA but positive by at least one of the confirmatory tests. Only two of these, both positive by ELISA, displayed evident signs of scrapie. In addition, 10 (6.6%) goats, which also included two clinical suspects, were negative on brain examination but had detectable PrP^Sc in lymphoid tissue. PrP^Sc was detected most frequently in the medial retropharyngeal lymph node (LN; 94.4% of all 18 cases) and palatine tonsil (88.9%). Abnormal behavior and circling or loss of balance when blindfolded were the best clinical discriminators for scrapie status. None of the goats that carried a single allele in the prion protein gene associated with increased resistance to scrapie (Q₂₁₁, K₂₂₂, S₁₄₆) were scrapie-positive, and the percentage of goats with these alleles was greater than expected from previous surveys. Significantly more goats that were scrapie-positive were isoleucine homozygous at codon 142 (II₁₄₂). The results indicate that the sensitivity of the applied screening test is poor in goats compared to the confirmatory tests as gold standard, particularly for asymptomatic animals. Sensitivity of surveillance could be improved by testing retropharyngeal LN or palatine tonsil in addition to brain.

Keywords: ELISA; classical scrapie; clinical diagnosis; goat; immunohistochemistry; prion; transmissible spongiform encephalopathy.