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Validation of a dual-probe quantitative reverse transcription polymerase chain reaction for rapid detection of spring viremia of carp virus

Authors
Park, Ji-YoonKim, Ji SuKim, Hyoung JunChoi, EunaKim, Do-HyungYun, DongbinKasai, HisaeNagata, JunJung, Tae SungKwon, Se Ryun
Issue Date
Jan-2026
Publisher
Elsevier BV
Keywords
Spring viremia of carp virus (SVCV); Dual-probe quantitative real-time polymerase; chain reaction (RT-qPCR); Validation
Citation
Aquaculture, v.612
Indexed
SCIE
SCOPUS
Journal Title
Aquaculture
Volume
612
URI
https://scholarworks.gnu.ac.kr/handle/sw.gnu/80084
DOI
10.1016/j.aquaculture.2025.743131
ISSN
0044-8486
1873-5622
Abstract
Accurate and sensitive disease diagnosis is crucial to prevent the global spread of spring viremia of carp virus (SVCV). In this study, we developed and validated a novel dual-probe quantitative reverse transcription polymerase chain reaction (RT-qPCR) method, which detects two distinct SVCV genomic sequences. The analytical sensitivity of the developed method was 6.2 copies of the SVCV plasmid (LoD95%). No cross-reactivity was observed with other viruses and fish cell lines. The diagnostic performance was further assessed using 550 koi carp (Cyprinus carpio) with a confirmed SVCV infection status. Compared to the conventional RT-PCR method, the dual-probe RT-PCR method diagnostic sensitivity (Dsn) and specificity (Dsp) of 100 % and 100 %, respectively. Additionally, when tested with 266 koi carp samples with an unconfirmed SVCV infection status, the novel method demonstrated a Dsn of 100 % and Dsp of 54.5 %, when compared to the of conventional RT-PCR method. No significant differences in inter- and intra-laboratory reproducibility were observed when performing PCRbased diagnosis using the novel method. Overall, the dual-probe RT-qPCR method targeting SVCV was found to be reliable tool for detecting the virus, suggesting its potential use in quarantine, surveillance, and monitoring programs.
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