Abstract
The utility of the VecTest antigen-capture assay to detect West Nile virus (WNV) in field-collected dead corvids was evaluated in Manitoba and Ontario, Canada, in 2001 and 2002. Swabs were taken from the oropharynx, cloaca, or both of 109 American Crows, 31 Blue Jays, 6 Common Ravens, and 4 Black-billed Magpies from Manitoba, and 255 American Crows and 28 Blue Jays from Ontario. The sensitivity and specificity of the antigen-capture assay were greatest for samples from American Crows; oropharyngeal swabs were more sensitive than cloacal swabs, and interlaboratory variation in the results was minimal. The sensitivity and specificity of the VecTest using oropharyngeal swabs from crows were 83.9% and 93.6%, respectively, for Manitoba samples and 83.3% and 95.8%, respectively, for Ontario birds. The VecTest antigen-capture assay on oropharyngeal secretions from crows is a reliable and rapid diagnostic test that appears suitable for incorporation into a WNV surveillance program.
Highlights
The utility of the VecTest antigen-capture assay to detect West Nile virus (WNV) in field-collected dead corvids was evaluated in Manitoba and Ontario, Canada, in 2001 and 2002
During 2001 and 2002, WNV was detected in avian tissues by using real-time TaqMan reverse transcription–polymerase chain reaction (RT-PCR), as described by Lanciotti et al [1]
The sensitivity and specificity of the VecTest assay for detecting WNV in oropharyngeal and cloacal swabs are presented in the Table
Summary
The utility of the VecTest antigen-capture assay to detect West Nile virus (WNV) in field-collected dead corvids was evaluated in Manitoba and Ontario, Canada, in 2001 and 2002. The sensitivity and specificity of the VecTest using oropharyngeal swabs from crows were 83.9% and 93.6%, respectively, for Manitoba samples and 83.3% and 95.8%, respectively, for Ontario birds. The ultimate goal of this study was to determine whether the VecTest assay could serve as a suitable alternative testing procedure for WNV dead bird surveillance. This goal was achieved by quantifying the sensitivity and specificity of this antigen-capture assay to detect WNV in corvids collected as part of routine dead bird surveillance programs in Manitoba and Ontario. The effect of storage conditions and duration of storage of swabs in grinding solution on the sensitivity of the assay and viability of virus was assessed
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