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Sensitivity of oral fluids for detecting influenza A virus in populations of vaccinated and non‐vaccinated pigs

Please cite this paper as: Romagosa et al. (2011) Sensitivity of oral fluids for detecting influenza A virus in populations of vaccinated and non‐vaccinated pigs. Influenza and Other Respiratory Viruses. Background/objective  We evaluated the sensitivity of PCR on oral fluids in detecting influenza...

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Autores principales: Romagosa, Anna, Gramer, Marie, Joo, Han Soo, Torremorell, Montserrat
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Blackwell Publishing Ltd 2011
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3203275/
https://www.ncbi.nlm.nih.gov/pubmed/21777397
http://dx.doi.org/10.1111/j.1750-2659.2011.00276.x
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author Romagosa, Anna
Gramer, Marie
Joo, Han Soo
Torremorell, Montserrat
author_facet Romagosa, Anna
Gramer, Marie
Joo, Han Soo
Torremorell, Montserrat
author_sort Romagosa, Anna
collection PubMed
description Please cite this paper as: Romagosa et al. (2011) Sensitivity of oral fluids for detecting influenza A virus in populations of vaccinated and non‐vaccinated pigs. Influenza and Other Respiratory Viruses. Background/objective  We evaluated the sensitivity of PCR on oral fluids in detecting influenza virus in vaccinated and non‐vaccinated pigs. Methods  Three‐week‐old influenza‐free pigs were divided into three groups: (i) control, non‐vaccinated, (ii) vaccinated with a commercial, heterologous vaccine, and (iii) vaccinated with an experimental, homologous vaccine. After vaccination, an influenza‐infected pig was placed in contact with each of the groups. Individual nasal swabs and pen oral fluids were collected daily. Viral RNA was tested for the presence of influenza by RRT‐PCR and virus isolation attempted from oral fluids. A pen was considered positive if at least one nasal swab was positive. Results  Based on nasal swab results, 43·8% of pens were detected positive but only 35% based on oral fluids. Overall sensitivity of oral fluids was 80%, and virus was isolated from 51% of RRT‐PCR‐positive oral fluids. The kappa coefficient for agreement (ĸ) between oral fluids and nasal swabs was 0·82. Among groups, ĸ was 1 (95% CI, 1–1), 0·74 (95% CI, 0·55–0·92), and 0·76 (95% CI, 0·5–1) for control, heterologous, and homologous‐vaccinated groups, respectively. There was less agreement when within pen prevalence was 10% or less. Probability of detecting influenza virus in oral fluids was 99% when within pen prevalence was higher than 18% and decreased to 69% when prevalence was 9%. Conclusions  Results indicated that pen‐based collection of oral fluids is a sensitive method to detect influenza even when within pen prevalence is low and when pigs have been vaccinated and highlight the potential use of oral fluids for influenza surveillance.
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spelling pubmed-32032752013-03-01 Sensitivity of oral fluids for detecting influenza A virus in populations of vaccinated and non‐vaccinated pigs Romagosa, Anna Gramer, Marie Joo, Han Soo Torremorell, Montserrat Influenza Other Respir Viruses Original Articles Please cite this paper as: Romagosa et al. (2011) Sensitivity of oral fluids for detecting influenza A virus in populations of vaccinated and non‐vaccinated pigs. Influenza and Other Respiratory Viruses. Background/objective  We evaluated the sensitivity of PCR on oral fluids in detecting influenza virus in vaccinated and non‐vaccinated pigs. Methods  Three‐week‐old influenza‐free pigs were divided into three groups: (i) control, non‐vaccinated, (ii) vaccinated with a commercial, heterologous vaccine, and (iii) vaccinated with an experimental, homologous vaccine. After vaccination, an influenza‐infected pig was placed in contact with each of the groups. Individual nasal swabs and pen oral fluids were collected daily. Viral RNA was tested for the presence of influenza by RRT‐PCR and virus isolation attempted from oral fluids. A pen was considered positive if at least one nasal swab was positive. Results  Based on nasal swab results, 43·8% of pens were detected positive but only 35% based on oral fluids. Overall sensitivity of oral fluids was 80%, and virus was isolated from 51% of RRT‐PCR‐positive oral fluids. The kappa coefficient for agreement (ĸ) between oral fluids and nasal swabs was 0·82. Among groups, ĸ was 1 (95% CI, 1–1), 0·74 (95% CI, 0·55–0·92), and 0·76 (95% CI, 0·5–1) for control, heterologous, and homologous‐vaccinated groups, respectively. There was less agreement when within pen prevalence was 10% or less. Probability of detecting influenza virus in oral fluids was 99% when within pen prevalence was higher than 18% and decreased to 69% when prevalence was 9%. Conclusions  Results indicated that pen‐based collection of oral fluids is a sensitive method to detect influenza even when within pen prevalence is low and when pigs have been vaccinated and highlight the potential use of oral fluids for influenza surveillance. Blackwell Publishing Ltd 2011-07-21 2012-03 /pmc/articles/PMC3203275/ /pubmed/21777397 http://dx.doi.org/10.1111/j.1750-2659.2011.00276.x Text en © 2011 Blackwell Publishing Ltd
spellingShingle Original Articles
Romagosa, Anna
Gramer, Marie
Joo, Han Soo
Torremorell, Montserrat
Sensitivity of oral fluids for detecting influenza A virus in populations of vaccinated and non‐vaccinated pigs
title Sensitivity of oral fluids for detecting influenza A virus in populations of vaccinated and non‐vaccinated pigs
title_full Sensitivity of oral fluids for detecting influenza A virus in populations of vaccinated and non‐vaccinated pigs
title_fullStr Sensitivity of oral fluids for detecting influenza A virus in populations of vaccinated and non‐vaccinated pigs
title_full_unstemmed Sensitivity of oral fluids for detecting influenza A virus in populations of vaccinated and non‐vaccinated pigs
title_short Sensitivity of oral fluids for detecting influenza A virus in populations of vaccinated and non‐vaccinated pigs
title_sort sensitivity of oral fluids for detecting influenza a virus in populations of vaccinated and non‐vaccinated pigs
topic Original Articles
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3203275/
https://www.ncbi.nlm.nih.gov/pubmed/21777397
http://dx.doi.org/10.1111/j.1750-2659.2011.00276.x
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