Development of a cost-effective method for capripoxvirus genotyping using snapback primer and dsDNA intercalating dye.

Development of a cost-effective method for capripoxvirus genotyping using snapback primer and dsDNA intercalating dye.

Sheep pox virus (SPPV), goat pox virus (GTPV) and lumpy skin disease virus (LSDV) are very closely related viruses of the Capripoxvirus (CaPV) genus of the Poxviridae family. They are responsible for sheep pox, goat pox and lumpy skin disease which affect sheep, goat and cattle, respectively. The ep...

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Main Authors: Esayas Gelaye, Charles Euloge Lamien, Roland Silber, Eeva S M Tuppurainen, Reingard Grabherr, Adama Diallo
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2013-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC3792100?pdf=render
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spelling doaj-c640f8b910ef4045b16e5e1412636d2c2020-11-24T21:16:20ZengPublic Library of Science (PLoS)PLoS ONE1932-62032013-01-01810e7597110.1371/journal.pone.0075971Development of a cost-effective method for capripoxvirus genotyping using snapback primer and dsDNA intercalating dye.Esayas GelayeCharles Euloge LamienRoland SilberEeva S M TuppurainenReingard GrabherrAdama DialloSheep pox virus (SPPV), goat pox virus (GTPV) and lumpy skin disease virus (LSDV) are very closely related viruses of the Capripoxvirus (CaPV) genus of the Poxviridae family. They are responsible for sheep pox, goat pox and lumpy skin disease which affect sheep, goat and cattle, respectively. The epidemiology of capripox diseases is complex, as some CaPVs are not strictly host-specific. Additionally, the three forms of the disease co-exist in many sub-Saharan countries which complicates the identification of the virus responsible for an outbreak. Genotyping of CaPVs using a low-cost, rapid, highly specific, and easy to perform method allows a swift and accurate identification of the causative agent and significantly assists in selecting appropriate control and eradication measures, such as the most suitable vaccine against the virus during the outbreaks. The objective of this paper is to describe the design and analytical performances of a new molecular assay for CaPV genotyping using unlabelled snapback primers in the presence of dsDNA intercalating EvaGreen dye. This assay was able to simultaneously detect and genotype CaPVs in 63 samples with a sensitivity and specificity of 100%. The genotyping was achieved by observing the melting temperature of snapback stems of the hairpins and those of the full-length amplicons, respectively. Fourteen CaPVs were genotyped as SPPVs, 25 as GTPVs and 24 as LSDVs. The method is highly pathogen specific and cross platform compatible. It is also cost effective as it does not use fluorescently labelled probes, nor require high-resolution melting curve analysis software. Thus it can be easily performed in diagnostic and research laboratories with limited resources. This genotyping method will contribute significantly to the early detection and genotyping of CaPV infection and to epidemiological studies.http://europepmc.org/articles/PMC3792100?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Esayas Gelaye
Charles Euloge Lamien
Roland Silber
Eeva S M Tuppurainen
Reingard Grabherr
Adama Diallo
spellingShingle Esayas Gelaye
Charles Euloge Lamien
Roland Silber
Eeva S M Tuppurainen
Reingard Grabherr
Adama Diallo
Development of a cost-effective method for capripoxvirus genotyping using snapback primer and dsDNA intercalating dye.
PLoS ONE
author_facet Esayas Gelaye
Charles Euloge Lamien
Roland Silber
Eeva S M Tuppurainen
Reingard Grabherr
Adama Diallo
author_sort Esayas Gelaye
title Development of a cost-effective method for capripoxvirus genotyping using snapback primer and dsDNA intercalating dye.
title_short Development of a cost-effective method for capripoxvirus genotyping using snapback primer and dsDNA intercalating dye.
title_full Development of a cost-effective method for capripoxvirus genotyping using snapback primer and dsDNA intercalating dye.
title_fullStr Development of a cost-effective method for capripoxvirus genotyping using snapback primer and dsDNA intercalating dye.
title_full_unstemmed Development of a cost-effective method for capripoxvirus genotyping using snapback primer and dsDNA intercalating dye.
title_sort development of a cost-effective method for capripoxvirus genotyping using snapback primer and dsdna intercalating dye.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2013-01-01
description Sheep pox virus (SPPV), goat pox virus (GTPV) and lumpy skin disease virus (LSDV) are very closely related viruses of the Capripoxvirus (CaPV) genus of the Poxviridae family. They are responsible for sheep pox, goat pox and lumpy skin disease which affect sheep, goat and cattle, respectively. The epidemiology of capripox diseases is complex, as some CaPVs are not strictly host-specific. Additionally, the three forms of the disease co-exist in many sub-Saharan countries which complicates the identification of the virus responsible for an outbreak. Genotyping of CaPVs using a low-cost, rapid, highly specific, and easy to perform method allows a swift and accurate identification of the causative agent and significantly assists in selecting appropriate control and eradication measures, such as the most suitable vaccine against the virus during the outbreaks. The objective of this paper is to describe the design and analytical performances of a new molecular assay for CaPV genotyping using unlabelled snapback primers in the presence of dsDNA intercalating EvaGreen dye. This assay was able to simultaneously detect and genotype CaPVs in 63 samples with a sensitivity and specificity of 100%. The genotyping was achieved by observing the melting temperature of snapback stems of the hairpins and those of the full-length amplicons, respectively. Fourteen CaPVs were genotyped as SPPVs, 25 as GTPVs and 24 as LSDVs. The method is highly pathogen specific and cross platform compatible. It is also cost effective as it does not use fluorescently labelled probes, nor require high-resolution melting curve analysis software. Thus it can be easily performed in diagnostic and research laboratories with limited resources. This genotyping method will contribute significantly to the early detection and genotyping of CaPV infection and to epidemiological studies.
url http://europepmc.org/articles/PMC3792100?pdf=render
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