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Cited 20 time in webofscience Cited 24 time in scopus
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Comparison of targeted next-generation sequencing for whole-genome sequencing of Hantaan orthohantavirus in Apodemus agrarius lung tissues

Authors
No, Jin SunKim, Won-KeunCho, SeungchanLee, Seung-HoKim, Jeong-AhLee, DaesangSong, Dong HyunGu, Se HunJeong, Seong TaeWiley, Michael R.Palacios, GustavoSong, Jin-Won
Issue Date
Nov-2019
Publisher
NATURE PUBLISHING GROUP
Citation
SCIENTIFIC REPORTS, v.9, no.1
Indexed
SCI
SCIE
SCOPUS
Journal Title
SCIENTIFIC REPORTS
Volume
9
Number
1
URI
https://scholarworks.korea.ac.kr/kumedicine/handle/2020.sw.kumedicine/1423
DOI
10.1038/s41598-019-53043-2
ISSN
2045-2322
Abstract
Orthohantaviruses, negative-sense single-strand tripartite RNA viruses, are a global public health threat. In humans, orthohantavirus infection causes hemorrhagic fever with renal syndrome or hantavirus cardiopulmonary syndrome. Whole-genome sequencing of the virus helps in identification and characterization of emerging or re-emerging viruses. Next-generation sequencing (NGS) is a potent method to sequence the viral genome, using molecular enrichment methods, from clinical specimens containing low virus titers. Hence, a comparative study on the target enrichment NGS methods is required for whole-genome sequencing of orthohantavirus in clinical samples. In this study, we used the sequence-independent, single-primer amplification, target capture, and amplicon NGS for whole-genome sequencing of Hantaan orthohantavirus (HTNV) from rodent specimens. We analyzed the coverage of the HTNV genome based on the viral RNA copy number, which is quantified by real-time quantitative PCR. Target capture and amplicon NGS demonstrated a high coverage rate of HTNV in Apodemus agrarius lung tissues containing up to 10(3)-10(4) copies/mu L of HTNV RNA. Furthermore, the amplicon NGS showed a 10-fold (10(2) copies/mu L) higher sensitivity than the target capture NGS. This report provides useful insights into target enrichment NGS for whole-genome sequencing of orthohantaviruses without cultivating the viruses.
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4. Research institute > Institute for Viral Diseases > 1. Journal Articles
1. Basic Science > Department of Microbiology > 1. Journal Articles

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