Use of real-time PCR to detect canine parvovirus in feces of free-ranging wolves

L. David Mech; Emily S. Almberg; Douglas Smith; Sagar Goyal; Randall S. Singer

doi:10.7589/0090-3558-48.2.473

Use of real-time PCR to detect canine parvovirus in feces of free-ranging wolves

L. David Mech, Emily S. Almberg, Douglas Smith, Sagar Goyal, Randall S. Singer

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8 Scopus citations

Abstract

Using real-time PCR, we tested 15 wolf (Canis lupus) feces from the Superior National Forest (SNF), Minnesota, USA, and 191 from Yellowstone National Park (YNP), USA, collected during summer and 13 during winter for canine parvovirus (CPV)-2 DNA. We also tested 20 dog feces for CPV-2 DNA. The PCR assay was 100%sensitive and specific with a minimum detection threshold of 104 50% tissue culture infective dose. Virus was detected in two winter specimens but none of the summer specimens. We suggest applying the technique more broadly especially with winter feces.

Original language	English (US)
Pages (from-to)	473-476
Number of pages	4
Journal	Journal of wildlife diseases
Volume	48
Issue number	2
DOIs	https://doi.org/10.7589/0090-3558-48.2.473
State	Published - 2012

Keywords

Canine parvovirus
Canis lupus
Feces
Real-time PCR
Wolf

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

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title = "Use of real-time PCR to detect canine parvovirus in feces of free-ranging wolves",

abstract = "Using real-time PCR, we tested 15 wolf (Canis lupus) feces from the Superior National Forest (SNF), Minnesota, USA, and 191 from Yellowstone National Park (YNP), USA, collected during summer and 13 during winter for canine parvovirus (CPV)-2 DNA. We also tested 20 dog feces for CPV-2 DNA. The PCR assay was 100%sensitive and specific with a minimum detection threshold of 104 50% tissue culture infective dose. Virus was detected in two winter specimens but none of the summer specimens. We suggest applying the technique more broadly especially with winter feces.",

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AU - Singer, Randall S.

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AB - Using real-time PCR, we tested 15 wolf (Canis lupus) feces from the Superior National Forest (SNF), Minnesota, USA, and 191 from Yellowstone National Park (YNP), USA, collected during summer and 13 during winter for canine parvovirus (CPV)-2 DNA. We also tested 20 dog feces for CPV-2 DNA. The PCR assay was 100%sensitive and specific with a minimum detection threshold of 104 50% tissue culture infective dose. Virus was detected in two winter specimens but none of the summer specimens. We suggest applying the technique more broadly especially with winter feces.

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Use of real-time PCR to detect canine parvovirus in feces of free-ranging wolves

Abstract

Keywords

UN SDGs

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