Journal ArticleDOI
A multiplex PCR for simultaneous detection and differentiation of North American serotypes of bluetongue and epizootic hemorrhagic disease viruses
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TLDR
The described multiplex RT-PCR-based assay could be used to facilitate rapid detection and differentiation of North American BTV and EHDV serotypes and to provide a valuable tool to study the epidemiology of these orbivirus infections in susceptible animal populations.Abstract:
In the present study, a multiplex RT-PCR-based assay for simultaneous detection and differentiation of North American serotypes of bluetongue (BT) virus (BTV) and epizootic hemorrhagic disease (EHD) virus (EHDV) in cell culture and clinical samples was developed. Two pairs of primers (B1 and B4) and (E1 and E4) were designed to hybridize to non-structural protein 1 (NS1) genomes of (BTV-11) and (EHDV-1), respectively. The multiplex PCR-based assay utilized a single tube-PCR amplification in which EHDV and BTV primers were used simultaneously in a multiplex format. The BTV primers generated a 790 base pair (bp) specific PCR product from RNA samples of North American BTV serotypes 2, 10, 11, 13 and 17; whereas EHDV serotypes 1 and 2 or total nucleic acid extract from non-infected baby hamster kidney (BHK) cells failed to demonstrate the 790bp specific BTV PCR product. Likewise, the EHDV primers produced a 387bp specific PCR product from RNA samples of EHDV serotypes 1 and 2, but not from BTV serotypes 2, 10, 11, 13, 17 or from total nucleic acid extract of BHK cell controls. Two pairs of nested primers (B2 and B3) and (E2 and E3), internal to the annealing sites of primers (B1and B4) and primers (E1 and E4), produced a 520bp specific BTV and a 224bp specific EHDV PCR product from BTV and EHDV first amplification products, respectively. These nested amplifications increased the sensitivity of the PCR assay and confirmed the specificity of the first amplified EHDV or BTV PCR products. The described multiplex RT-PCR-based assay could be used to facilitate rapid detection and differentiation of North American BTV and EHDV serotypes and to provide a valuable tool to study the epidemiology of these orbivirus infections in susceptible animal populations.read more
Citations
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Journal ArticleDOI
Bluetongue virus detection by two real-time RT-qPCRs targeting two different genomic segments.
TL;DR: Two laboratories joined forces to develop and validate two new RT-qPCRs detecting and amplifying BTV segments 1 and 5, which are complementary and could be used in parallel to confirm the diagnosis of a possible new introduction of BTV.
Journal ArticleDOI
Development and initial evaluation of a real-time RT-PCR assay to detect bluetongue virus genome segment 1
Andrew Shaw,Paul Monaghan,H.O. Alpar,Simon J. Anthony,Karin E. Darpel,Carrie Batten,Annalisa Guercio,G. Alimena,Maria Vitale,K. Bankowska,Simon Carpenter,H. Jones,C.A.L. Oura,Donald P. King,Heather Elliott,P. S. Mellor,Peter P. C. Mertens +16 more
TL;DR: A real-time RT-PCR assay that targets the highly conserved genome segment 1 (encoding the viral polymerase--VP1) that can be used to detect all of the 24 serotypes, as well as geographic variants (different topotypes) within individual serotypes of BTV.
Journal ArticleDOI
Bluetongue in northern Europe.
Etienne Thiry,Claude Saegerman,Hugues Guyot,Philippe Kirten,Bertrand Losson,Frédéric Rollin,Michèle Bodmer,Guy Czaplicki,Jean-François Toussaint,Kris De Clercq,Jean-Marie Dochy,J. Dufey,Jean-Luc Gilleman,Karl Messeman +13 more
TL;DR: The first cases of bluetongue were confirmed by the detection of specific antibodies by elisa and by real-time reverse transcriptase-pcr performed on whole blood as discussed by the authors.
Bluetongue in northern Europe.
TL;DR: Belgium notified its first cases of bluetongue on August 18 and suspicions of the disease were confirmed by the detection of specific antibodies by elisa and by real-time reverse transcriptase-pcr performed on whole blood.
Journal ArticleDOI
A duplex RT-PCR assay for detection of genome segment 7 (VP7 gene) from 24 BTV serotypes
Simon J. Anthony,H. Jones,Karin E. Darpel,Heather Elliott,Sushila Maan,A R Samuel,P. S. Mellor,Peter P. C. Mertens +7 more
TL;DR: The assay reliably amplified Seg-7 from any of the BTV strains tested, including isolates of the 24 BTV serotypes and isolates from different geographic origins, and no cross-reactions were detected with members of closely related Orbivirus species.
References
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Book ChapterDOI
The International Committee on Taxonomy of Viruses
Frederick A. Murphy,Claude M. Fauquet,David H. L. Bishop,Said A. Ghabrial,Audrey W. Jarvis,Giovanni P. Martelli,Michael Mayo,Max D. Summers +7 more
Journal ArticleDOI
Progress in Clinical and Biological Research
TL;DR: All with an interest in tumours will find something to stimulate them in this book but even these items are to some extent outweighed by the insight given into the thoughts and policies of this fascinating country.
Journal ArticleDOI
Physicochemical and morphological relationships of some arthropod-borne viruses to bluetongue virus--a new taxonomic group. Physiocochemical and serological studies.
TL;DR: Several arthropod-borne viruses were grouped on the basis of relative stability to lipid solvents and sodium deoxycholate, lability at pH 3.0, and lack of antigenic relationship to major arbovirus serologic groups A, B, and Bunyamwera, distinguished from reoviruses by acid lability, slight solvent sensitivity, and serology.
Journal ArticleDOI
A virus-induced epizootic hemorrhagic disease of the virginia white-tailed deer (odocoileus virginianus)
TL;DR: A circumscribed natural outbreak of a highly fatal disease of deer, which the authors have designated epizootic hemorrhagic disease (EHD), has been studied and it has proven readily transmissible in deer but not in other experimental or domestic animals tested, nor in embryonating eggs or deer kidney cell cultures.