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Development of an RT-LAMP-CRISPR/ Cas12a assay for rapid and specific detection of Bandavirus dabieense

Authors
Song, Bo SeungBaek, Yun HeeKim, Eun-HaKwon, Hyeok-IlKim, Ah-HyeonLee, Si-HyunSon, Yu-BinKim, Soo-HyeonSong, Min-SukChoi, Young KiPark, Su-Jin
Issue Date
Nov-2025
Publisher
한국미생물학회
Keywords
RT-LAMP associated CRISPR Cas12a; Bandavirus dabieense; diagnosis; SFTS
Citation
Journal of Microbiology, v.63, no.11
Indexed
SCIE
SCOPUS
KCI
Journal Title
Journal of Microbiology
Volume
63
Number
11
URI
https://scholarworks.gnu.ac.kr/handle/sw.gnu/81580
DOI
10.71150/jm.2506013
ISSN
1225-8873
1976-3794
Abstract
Bandavirus dabieense, a single-stranded RNA virus, is the causative agent of severe fever with thrombocytopenia syndrome (SFTS), a disease associated with high fatality rates. Early and accurate diagnosis is essential for improving clinical outcomes, particularly given the limited therapeutic options and high mortality rates associated with SFTS. However, while highly sensitive, conventional diagnostic methods such as PCR and qRT-PCR require specialized laboratory facilities and trained personnel, making them impractical for rapid detection in resource-limited settings. To address these challenges, we developed a rapid and highly sensitive assay for Bandavirus dabieense detection by integrating reverse transcription loop-mediated isothermal amplification (RT-LAMP) with CRISPR/Cas12a technology. LAMP primers and guide RNA sequences were designed to target the L gene, ensuring broad detection across viral genotypes. The optimized assay demonstrated a detection limit of 5 RNA copies per reaction, showing more sensitivity than qRT-PCR, and exhibited 100% concordance with qRT-PCR results in clinical samples. Given its speed, accuracy, and field applicability, this LAMP-CRISPR/Cas12a-based assay represents a promising diagnostic tool for early SFTSV detection, particularly in resource-constrained environments where conventional molecular diagnostics are not readily available.
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자연과학대학 (생명과학부)
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