Rapid Detection of Peste des Petits Ruminants Virus (PPRV) Nucleic Acid Using a Novel Low-Cost Reverse Transcription Loop-Mediated Isothermal Amplification (RT-LAMP) Assay for Future Use in Nascent PPR Eradication Programme.
Animals
DNA Primers
/ genetics
DNA, Viral
/ isolation & purification
Disease Outbreaks
/ prevention & control
Eye
/ virology
Goat Diseases
/ diagnosis
Goats
/ virology
Nose
/ virology
Nucleic Acid Amplification Techniques
/ methods
Nucleocapsid Proteins
/ genetics
Pathology, Molecular
/ methods
Peste-des-Petits-Ruminants
/ blood
Peste-des-petits-ruminants virus
/ isolation & purification
Reverse Transcription
Sensitivity and Specificity
Sheep
Sheep Diseases
/ diagnosis
Temperature
PPRV
RT-LAMP
diagnostics
eradication programme
pen side
rapid detection
Journal
Viruses
ISSN: 1999-4915
Titre abrégé: Viruses
Pays: Switzerland
ID NLM: 101509722
Informations de publication
Date de publication:
31 07 2019
31 07 2019
Historique:
received:
21
06
2019
revised:
26
07
2019
accepted:
30
07
2019
entrez:
3
8
2019
pubmed:
3
8
2019
medline:
26
9
2020
Statut:
epublish
Résumé
Peste des petits ruminants (PPR) is a disease of small ruminants caused by peste des petits ruminants virus (PPRV), and is endemic in Asia, the Middle East and Africa. Effective control combines the application of early warning systems, accurate laboratory diagnosis and reporting, animal movement restrictions, suitable vaccination and surveillance programs, and the coordination of all these measures by efficient veterinary services. Molecular assays, including conventional reverse transcription-polymerase chain reaction (RT-PCR) and real-time RT-PCR (RT-qPCR) have improved the sensitivity and rapidity of diagnosing PPR. However, currently these assays are only performed within laboratory settings; therefore, the development of field diagnostics for PPR would improve the fast implementation of control policies, particularly when PPR has been targeted to be eradicated by 2030. Loop-mediated isothermal amplification (LAMP) assays are simple to use, rapid, and have sensitivity and specificity within the range of RT-qPCR; and can be performed in the field using disposable consumables and portable equipment. This study describes the development of a novel RT-LAMP assay for the detection of PPRV nucleic acid by targeting the N-protein gene. The RT-LAMP assay was evaluated using cell culture propagated PPRVs, field samples from clinically infected animals and samples from experimentally infected animals encompassing all four lineages (I-IV) of PPRV. The test displayed 100% concordance with RT-qPCR when considering an RT-qPCR cut-off value of C
Identifiants
pubmed: 31370329
pii: v11080699
doi: 10.3390/v11080699
pmc: PMC6723471
pii:
doi:
Substances chimiques
DNA Primers
0
DNA, Viral
0
Nucleocapsid Proteins
0
Types de publication
Journal Article
Research Support, Non-U.S. Gov't
Langues
eng
Sous-ensembles de citation
IM
Subventions
Organisme : Biotechnology and Biological Sciences Research Council
ID : BBS/E/I/00007031
Pays : United Kingdom
Organisme : Biotechnology and Biological Sciences Research Council
ID : BBS/E/I/00007036
Pays : United Kingdom
Organisme : Biotechnology and Biological Sciences Research Council
ID : BBS/E/I/00007037
Pays : United Kingdom
Organisme : Biotechnology and Biological Sciences Research Council
ID : BB/L004801/1, BB/L004801/1, BBS/E/I/00007036 and BBS/E/I/00007037
Pays : United Kingdom
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