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Peer-reviewed veterinary case report

Development of a two-step SYBR Green I based real time RT-PCR assay for detecting and quantifying peste des petits ruminants virus in clinical samples.

Journal:
Journal of virological methods
Year:
2014
Authors:
Abera, Tsegalem & Thangavelu, Ardhanary
Affiliation:
Department of Veterinary Microbiology · India
Species:
dog

Plain-English summary

Researchers developed a new test to detect and measure the Peste des petits ruminants virus (PPRV), which affects small ruminants like sheep and goats. They found that this test was very specific, meaning it didn't mistakenly identify other similar viruses, and it could detect very low amounts of the virus in samples. When they tested 36 samples suspected of having PPRV, the new test identified the virus in 32 of them, while a traditional test only found it in 19. This shows that the new test is more effective at finding the virus. Overall, the new test is reliable and sensitive for detecting PPRV.

Abstract

A two-step SYBR Green I based real time RT-PCR targeting the matrix (M) gene of Peste des petits ruminants virus (PPRV) was developed. The specificity of the assay was assessed against viral nucleic acid extracted from a range of animal viruses of clinical and structural similarities to PPRV including canine distemper virus, measles virus, bluetongue virus and Newcastle disease virus. But none of the viruses and no template control showed an amplification signal. Sensitivity of the same assay was assessed based on plasmid DNA copy number and with respect to infectivity titre. The lower detection limit achieved was 2.88 plasmid DNA copies/μl with corresponding Ct value of 35.93. Based on tissue culture infectivity titre the lower detection limits were 0.0001TCID50/ml and 1TCID50/ml for the SYBR green I based real time RT-PCR and conventional RT-PCR, respectively. The calculated coefficient of variations values for intra- and inter-assay variability were low, ranging from 0.21% to 1.83% and 0.44% to 1.97%, respectively. The performance of newly developed assay was evaluated on a total of 36 clinical samples suspected of PPR and compared with conventional RT-PCR. The SYBR Green I based real time RT-PCR assay detected PPRV in 32 (88.8%) of clinical samples compared to 19 (52.7%) by conventional RT-PCR. Thus, the two-step SYBR Green I based real time RT-PCR assay targeting the M gene of PPRV reported in this study was highly sensitive, specific and reproducible for detection and quantitation of PPRV nucleic acids.

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Original publication: https://pubmed.ncbi.nlm.nih.gov/25194891/