Evaluation of Non-Invasive Sampling Techniques for the Molecular Surveillance of Equid Herpesviruses in Yearling Horses-Reference-Cited by-同舟云学术

Evaluation of Non-Invasive Sampling Techniques for the Molecular Surveillance of Equid Herpesviruses in Yearling Horses

Published:2024-07-07 Issue:7 Volume:16 Page:1091
ISSN:1999-4915
Container-title:Viruses
language:en
Short-container-title:Viruses

Author:

Khan Amjad¹²^ORCID,Olajide Edward¹,Friedrich Madeline³,Holt Anna³,Goehring Lutz S.¹

Affiliation:

1. Department of Veterinary Science, Martin-Gatton College of Agriculture, Food and the Environment, University of Kentucky, Lexington, KY 40506, USA

2. Department of Public Health & Nutrition, University of Haripur, Haripur 22600, Pakistan

3. College of Veterinary Medicine, Lincoln Memorial University, Harrogate, TN 37752-8245, USA

Abstract

Background: Equid alphaherpesvirus 1 (EHV-1) is a highly contagious respiratory tract pathogen of horses, and infection may be followed by myeloencephalopathy or abortion. Surveillance and early detection have focused on PCR assays using less tolerated nasal swabs. Here, we assess non-invasive non-contact sampling techniques as surveillance tools in naturally equid gammaherpesvirus 2-shedding horses as surrogates for EHV-1. Methods: Horses were individually housed for 10 h periods on 2 consecutive days. Sampling included nasal swabs, nostril wipes, environmental swabs, droplet-catching devices, and air sampling. The latter was completed via two strategies: a combined air sample collected while going from horse to horse and a collective air sample collected at a stationary central point for 6 h. Samples were screened through quantitative PCR and digital PCR. Results: Nine horses on day 1 and 11 horses on day 2 were positive for EHV-1; overall, 90.9% of the nostril wipes, 81.8% of the environmental surfaces, and 90.9% of the droplet-catching devices were found to be positive. Quantitative analysis showed that the mean DNA copies detection per cm2 of nostril wipe sampled concentration (4.3 × 105 per day) was significantly (p < 0.05) comparable to that of nasal swabs (3.6 × 105 per day) followed by environmental swabs (4.3 × 105 per day) and droplet catchers (3.5 × 103 per day), respectively. Overall, 100% of the air samples collected were positive on both qPCR and dPCR. In individual air samples, a mean concentration of 1.0 × 104 copies of DNA were detected in per m3 air sampled per day, while in the collective air samples, the mean concentration was 1.1 × 103. Conclusions: Environmental samples look promising in replacing direct contact sampling. Environmental and air sampling could become efficient surveillance tools at equestrian events; however, it needs threshold calculations for minimum detection levels.

Funder

INTERNATIONAL EQUESTRIAN FEDERATION (FEI) Lausanne, Switzerland

Publisher

MDPI AG

Link

https://www.mdpi.com/1999-4915/16/7/1091/pdf

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