Development and evaluation of a one-step multiplex real-time TaqMan® RT-qPCR assay for the detection and genotyping of equine G3 and G14 rotaviruses in fecal samples

Carossino, Mariano; Barrandeguy, Maria Edith; Erol, Erdal; Li, Yanqiu; Balasuriya, Udeni B.R.

resumen

Resumen

Background: Equine rotavirus A (ERVA) is the leading cause of diarrhea in neonatal foals and has a negative impact on equine breeding enterprises worldwide. Among ERVA strains infecting foals, the genotypes G3P[12] and G14P[12] are the most prevalent, while infections by strains with other genomic arrangements are infrequent. The identification of circulating strains of ERVA is critical for diagnostic and surveillance purposes, as well as to understand their molecular epidemiology. Current genotyping methods available for ERVA and rotaviruses affecting other animal species rely on Sanger sequencing and are significantly time-consuming, costly and labor intensive. Here, we developed the first one-step multiplex TaqMan® real-time reverse transcription polymerase chain reaction (RT-qPCR) assay targeting the NSP3 and VP7 genes of ERVA G3 and G14 genotypes for the rapid detection and G-typing directly from fecal specimens. Methods: A one-step multiplex TaqMan® RT-qPCR assay targeting the NSP3 and VP7 genes of ERVA G3 and G14 genotypes was designed. The analytical sensitivity was assessed using serial dilutions of in vitro transcribed RNA containing the target sequences while the analytical specificity was determined using RNA and DNA derived from a panel of group A rotaviruses along with other equine viruses and bacteria. The clinical performance of this multiplex assay was evaluated using a panel of 177 fecal samples and compared to a VP7-specific standard RT-PCR assay and Sanger sequencing. Limits of detection (LOD), sensitivity, specificity, and agreement were determined. Results: The multiplex G3 and G14 VP7 assays demonstrated high specificity and efficiency, with perfect linearity. A 100-fold difference in their analytical sensitivity was observed when compared to the singleplex assays; however, this difference did not have an impact on the clinical performance. Clinical performance of the multiplex RT-qPCR assay demonstrated that this assay had a high sensitivity/specificity for every target (100% for NSP3, > 90% for G3 VP7 and > 99% for G14 VP7, respectively) and high overall agreement (> 98%) compared to conventional RT-PCR and sequencing. Conclusions: This new multiplex RT-qPCR assay constitutes a useful, very reliable tool that could significantly aid in the rapid detection and G-typing of ERVA strains circulating in the field. [Cerrar]

dc.contributor.author	Carossino, Mariano
dc.contributor.author	Barrandeguy, Maria Edith
dc.contributor.author	Erol, Erdal
dc.contributor.author	Li, Yanqiu
dc.contributor.author	Balasuriya, Udeni B.R.
dc.date.accessioned	2019-05-17T14:31:34Z
dc.date.available	2019-05-17T14:31:34Z
dc.date.issued	2019-04
dc.identifier.issn	1743-422X
dc.identifier.other	https://doi.org/10.1186/s12985-019-1149-1
dc.identifier.uri	https://virologyj.biomedcentral.com/articles/10.1186/s12985-019-1149-1
dc.identifier.uri	http://hdl.handle.net/20.500.12123/5143
dc.description.abstract	Background: Equine rotavirus A (ERVA) is the leading cause of diarrhea in neonatal foals and has a negative impact on equine breeding enterprises worldwide. Among ERVA strains infecting foals, the genotypes G3P[12] and G14P[12] are the most prevalent, while infections by strains with other genomic arrangements are infrequent. The identification of circulating strains of ERVA is critical for diagnostic and surveillance purposes, as well as to understand their molecular epidemiology. Current genotyping methods available for ERVA and rotaviruses affecting other animal species rely on Sanger sequencing and are significantly time-consuming, costly and labor intensive. Here, we developed the first one-step multiplex TaqMan® real-time reverse transcription polymerase chain reaction (RT-qPCR) assay targeting the NSP3 and VP7 genes of ERVA G3 and G14 genotypes for the rapid detection and G-typing directly from fecal specimens. Methods: A one-step multiplex TaqMan® RT-qPCR assay targeting the NSP3 and VP7 genes of ERVA G3 and G14 genotypes was designed. The analytical sensitivity was assessed using serial dilutions of in vitro transcribed RNA containing the target sequences while the analytical specificity was determined using RNA and DNA derived from a panel of group A rotaviruses along with other equine viruses and bacteria. The clinical performance of this multiplex assay was evaluated using a panel of 177 fecal samples and compared to a VP7-specific standard RT-PCR assay and Sanger sequencing. Limits of detection (LOD), sensitivity, specificity, and agreement were determined. Results: The multiplex G3 and G14 VP7 assays demonstrated high specificity and efficiency, with perfect linearity. A 100-fold difference in their analytical sensitivity was observed when compared to the singleplex assays; however, this difference did not have an impact on the clinical performance. Clinical performance of the multiplex RT-qPCR assay demonstrated that this assay had a high sensitivity/specificity for every target (100% for NSP3, > 90% for G3 VP7 and > 99% for G14 VP7, respectively) and high overall agreement (> 98%) compared to conventional RT-PCR and sequencing. Conclusions: This new multiplex RT-qPCR assay constitutes a useful, very reliable tool that could significantly aid in the rapid detection and G-typing of ERVA strains circulating in the field.	eng
dc.format	application/pdf	es_AR
dc.language.iso	eng	es_AR
dc.publisher	BMC	es_AR
dc.rights	info:eu-repo/semantics/openAccess	es_AR
dc.rights.uri	http://creativecommons.org/licenses/by-nc-sa/4.0/
dc.source	Virology Journal 16 (1) : 49 (Abril 2019)	es_AR
dc.subject	Rotavirus	es_AR
dc.subject	Diarrhoea	eng
dc.subject	Diarrea	es_AR
dc.subject	PCR	es_AR
dc.subject	Genotypes	eng
dc.subject	Genotipos	es_AR
dc.subject	Horses	eng
dc.subject	Caballos	es_AR
dc.subject	Foals	eng
dc.subject	Potro	es_AR
dc.subject.other	Rotavirus A	es_AR
dc.subject.other	Equine rotavirus	eng
dc.subject.other	Rotavirus equino	es_AR
dc.title	Development and evaluation of a one-step multiplex real-time TaqMan® RT-qPCR assay for the detection and genotyping of equine G3 and G14 rotaviruses in fecal samples	es_AR
dc.type	info:ar-repo/semantics/artículo	es_AR
dc.type	info:eu-repo/semantics/article	es_AR
dc.type	info:eu-repo/semantics/publishedVersion	es_AR
dc.rights.license	Creative Commons Attribution-NonCommercial-ShareAlike 4.0 International (CC BY-NC-SA 4.0)
dc.description.origen	Instituto de Virología	es_AR
dc.description.fil	Fil: Carossino, Mariano. Louisiana State University. School of Veterinary Medicine. Louisiana Animal Disease Diagnostic Laboratory and Department of Pathobiological Sciences; Estados Unidos. Universidad del Salvador. Escuela de Veterinaria; Argentina	es_AR
dc.description.fil	Fil: Barrandeguy, Maria Edith. Instituto Nacional de Tecnología Agropecuaria (INTA). Instituto de Virología; Argentina. Universidad del Salvador. Escuela de Veterinaria; Argentina	es_AR
dc.description.fil	Fil: Erol, Erdal. University of Kentucky. Department of Veterinary Science. University of Kentucky Veterinary Diagnostic Laboratory; Estados Unidos	es_AR
dc.description.fil	Fil: Li, Yanqiu. University of Kentucky. Department of Veterinary Science. Maxwell H. Gluck Equine Research Center; Estados Unidos	es_AR
dc.description.fil	Fil: Balasuriya, Udeni B. R. Louisiana State University. School of Veterinary Medicine. Louisiana Animal Disease Diagnostic Laboratory and Department of Pathobiological Sciences; Estados Unidos	es_AR
dc.subtype	cientifico

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