Equivalence of Self- and Staff-Collected Nasal Swabs for the Detection of Viral Respiratory Pathogens

BACKGROUND: The need for the timely collection of diagnostic biosamples during symptomatic episodes represents a major obstacle to large-scale studies on acute respiratory infection (ARI) epidemiology. This may be circumvented by having the participants collect their own nasal swabs. We compared sel...

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Autores principales: Akmatov, Manas K., Gatzemeier, Anja, Schughart, Klaus, Pessler, Frank
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2012
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3498275/
https://www.ncbi.nlm.nih.gov/pubmed/23155387
http://dx.doi.org/10.1371/journal.pone.0048508
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author Akmatov, Manas K.
Gatzemeier, Anja
Schughart, Klaus
Pessler, Frank
author_facet Akmatov, Manas K.
Gatzemeier, Anja
Schughart, Klaus
Pessler, Frank
author_sort Akmatov, Manas K.
collection PubMed
description BACKGROUND: The need for the timely collection of diagnostic biosamples during symptomatic episodes represents a major obstacle to large-scale studies on acute respiratory infection (ARI) epidemiology. This may be circumvented by having the participants collect their own nasal swabs. We compared self- and staff-collected swabs in terms of swabbing quality and detection of viral respiratory pathogens. METHODOLOGY/PRINCIPAL FINDINGS: We conducted a prospective study among employees of our institution during the ARI season 2010/2011 (December-March). Weekly emails were sent to the participants (n = 84), reminding them to come to the study center in case of new symptoms. The participants self-collected an anterior nasal swab from one nostril, and trained study personnel collected one from the other nostril. The participants self-collected another two swabs (one from each nostril) on a subsequent day. Human β-actin DNA concentration was determined in the swabs as a quality control. Viral respiratory pathogens were detected by multiplex RT-PCR (Seeplex RV15 kit, Seegene, Eschborn, Germany). Of 84 participants, 56 (67%) reported at least one ARI episode, 18 participants two, and one participant three. Self-swabbing was highly accepted by the participants. The amount of β-actin DNA per swab was higher in the self- than in the staff-collected swabs (p = 0.008). β-actin concentration was lower in the self-swabs collected on day 1 than in those collected on a subsequent day (p<0.0001). A respiratory viral pathogen was detected in 31% (23/75) of staff- and in 35% (26/75) of self-collected swabs (p = 0.36). With both approaches, the most frequently identified pathogens were human rhinoviruses A/B/C (12/75 swabs, 16%) and human coronavirus OC43 (4/75 swabs, 5%). There was almost perfect agreement between self- and staff-collected swabs in terms of pathogen detection (agreement = 93%, kappa = 0.85, p<0.0001). CONCLUSIONS/SIGNIFICANCE: Nasal self-swabbing for identification of viral ARI pathogens proved to be equivalent to staff-swabbing in this population in terms of acceptance and pathogen detection.
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spelling pubmed-34982752012-11-15 Equivalence of Self- and Staff-Collected Nasal Swabs for the Detection of Viral Respiratory Pathogens Akmatov, Manas K. Gatzemeier, Anja Schughart, Klaus Pessler, Frank PLoS One Research Article BACKGROUND: The need for the timely collection of diagnostic biosamples during symptomatic episodes represents a major obstacle to large-scale studies on acute respiratory infection (ARI) epidemiology. This may be circumvented by having the participants collect their own nasal swabs. We compared self- and staff-collected swabs in terms of swabbing quality and detection of viral respiratory pathogens. METHODOLOGY/PRINCIPAL FINDINGS: We conducted a prospective study among employees of our institution during the ARI season 2010/2011 (December-March). Weekly emails were sent to the participants (n = 84), reminding them to come to the study center in case of new symptoms. The participants self-collected an anterior nasal swab from one nostril, and trained study personnel collected one from the other nostril. The participants self-collected another two swabs (one from each nostril) on a subsequent day. Human β-actin DNA concentration was determined in the swabs as a quality control. Viral respiratory pathogens were detected by multiplex RT-PCR (Seeplex RV15 kit, Seegene, Eschborn, Germany). Of 84 participants, 56 (67%) reported at least one ARI episode, 18 participants two, and one participant three. Self-swabbing was highly accepted by the participants. The amount of β-actin DNA per swab was higher in the self- than in the staff-collected swabs (p = 0.008). β-actin concentration was lower in the self-swabs collected on day 1 than in those collected on a subsequent day (p<0.0001). A respiratory viral pathogen was detected in 31% (23/75) of staff- and in 35% (26/75) of self-collected swabs (p = 0.36). With both approaches, the most frequently identified pathogens were human rhinoviruses A/B/C (12/75 swabs, 16%) and human coronavirus OC43 (4/75 swabs, 5%). There was almost perfect agreement between self- and staff-collected swabs in terms of pathogen detection (agreement = 93%, kappa = 0.85, p<0.0001). CONCLUSIONS/SIGNIFICANCE: Nasal self-swabbing for identification of viral ARI pathogens proved to be equivalent to staff-swabbing in this population in terms of acceptance and pathogen detection. Public Library of Science 2012-11-14 /pmc/articles/PMC3498275/ /pubmed/23155387 http://dx.doi.org/10.1371/journal.pone.0048508 Text en © 2012 Akmatov et al http://creativecommons.org/licenses/by/4.0/ This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.
spellingShingle Research Article
Akmatov, Manas K.
Gatzemeier, Anja
Schughart, Klaus
Pessler, Frank
Equivalence of Self- and Staff-Collected Nasal Swabs for the Detection of Viral Respiratory Pathogens
title Equivalence of Self- and Staff-Collected Nasal Swabs for the Detection of Viral Respiratory Pathogens
title_full Equivalence of Self- and Staff-Collected Nasal Swabs for the Detection of Viral Respiratory Pathogens
title_fullStr Equivalence of Self- and Staff-Collected Nasal Swabs for the Detection of Viral Respiratory Pathogens
title_full_unstemmed Equivalence of Self- and Staff-Collected Nasal Swabs for the Detection of Viral Respiratory Pathogens
title_short Equivalence of Self- and Staff-Collected Nasal Swabs for the Detection of Viral Respiratory Pathogens
title_sort equivalence of self- and staff-collected nasal swabs for the detection of viral respiratory pathogens
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3498275/
https://www.ncbi.nlm.nih.gov/pubmed/23155387
http://dx.doi.org/10.1371/journal.pone.0048508
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