Pepin BJ, Kittawornrat A, Liu F, Gauger PC, Harmon K, Abate S, Main R, Garton C, Hargrove J, Rademacher C, Ramirez A, Zimmerman J. Comparison of specimens for detection of porcine reproductive and
respiratory syndrome virus infection in boar studs. Transbound Emerg Dis. 2015
Jun;62(3):295-304. doi: 10.1111/tbed.12135. Epub 2013 Jul 30.
Abstract
Porcine
reproductive and respiratory syndrome virus (PRRSV)-contaminated semen from
boars is a route of transmission to females, and early detection of PRRSV
infection in boars is a key component in sow farm biosecurity. The purpose of
this study was to determine the optimum diagnostic specimen(s) for the
detection of acute PRRSV infection in boars. Individually housed boars (n = 15)
were trained for semen and oral fluid collection and then vaccinated with a
commercial PRRSV modified live virus vaccine. Starting on the day of
vaccination and for 14 days thereafter, oral fluid specimens were collected
daily from all boars. The 15 boars were subdivided into three groups of 5, and
serum, blood swabs and 'frothy saliva' were collected at the time of semen
collection on a 3-day rotation. Frothy saliva, derived from the submandibular
salivary gland, is produced by aroused boars. Semen was centrifuged, and semen
supernatant and cell fractions were tested separately. All samples were
randomly ordered and then tested by PRRSV real-time quantitative reverse-transcription
polymerase chain reaction assay (rRT-PCR) and PRRSV antibody ELISA. In this
study, a comparison of serum, blood swab, and oral fluid rRT-PCR results found
no statistically significant differences in the onset of detection or
proportion of positives, but serum was numerically superior to oral fluids for
early detection. Serum and oral fluid provided identical rRT-PCR results at ≥ 5
day post-vaccination. Likewise, the onset of detection of PRRSV antibody in
serum, oral fluid and frothy saliva was statistically equivalent, with serum
results again showing a numerical advantage. These results showed that the
highest assurance of providing PRRSV-negative semen to sow farms should be
based on rRT-PCR testing of serum collected at the time of semen collection.
This approach can be augmented with oral fluid sampling from a random selection
of uncollected boars to provide for statistically valid surveillance of the
boar stud.
© 2013
Blackwell Verlag GmbH.
KEYWORDS:
PRRSV; boar; oral fluid;
semen; serum; surveillance
PMID:
23895185 [PubMed - in process]
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