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The virome of acute respiratory diseases in individuals at risk of zoonotic infections

Kha Tu N.T. Doctoral School in Health Sciences, Faculty of Medicine, University of Helsinki, Helsinki, 00014, Finland|
VIZIONS Consortium | van Tan L. | Baker S. | Vapalahti O. | Virtala A.-M.K. | Delwart E. | Thwaites G. | Deng X. | Thu Ha L.T. Cambridge Institute of Therapeutic Immunology & Infectious Disease (CITIID), Department of Medicine, University of Cambridge, Cambridge, CB2 0QQ, United Kingdom| Han D.A. Virology and Immunology, HUSLAB, Helsinki University Hospital, Helsinki, 00029, Finland| Huong D.T. Department of Veterinary Biosciences, Faculty of Veterinary Medicine, University of Helsinki, Helsinki, 00014, Finland| Trung Nghia H.D. Vitalant Research Institute, San Francisco, CA 94118, United States| van Doorn H.R. Department of Laboratory Medicine, University of California, San Francisco, CA 94143, United States| Thanh Tam P.T. Centre for Tropical Medicine and Global Health, Nuffield Department of Medicine, University of Oxford, Oxford, OX3 7LG, United Kingdom| Phuc T.M. Oxford University Clinical Research Unit, Ha Noi, 8000, Viet Nam| Han Ny N.T. Dong Thap Provincial Center for Disease Control, Cao Lanh, Dong Thap Province, 660273, Viet Nam| Thu Hong N.T. Oxford University Clinical Research Unit, Ho Chi Minh City, 7000, Viet Nam|

Viruses Số 9, năm 2020 (Tập 12, trang -)

ISSN: 19994915

ISSN: 19994915

DOI: 10.3390/v12090960

Tài liệu thuộc danh mục: ISI, Scopus

Article

English

Tóm tắt tiếng anh
The ongoing coronavirus disease 2019 (COVID-19) pandemic emphasizes the need to actively study the virome of unexplained respiratory diseases. We performed viral metagenomic next-generation sequencing (mNGS) analysis of 91 nasal-throat swabs from individuals working with animals and with acute respiratory diseases. Fifteen virus RT-PCR-positive samples were included as controls, while the other 76 samples were RT-PCR negative for a wide panel of respiratory pathogens. Eukaryotic viruses detected by mNGS were then screened by PCR (using primers based on mNGS-derived contigs) in all samples to compare viral detection by mNGS versus PCR and assess the utility of mNGS in routine diagnostics. mNGS identified expected human rhinoviruses, enteroviruses, influenza A virus, coronavirus OC43, and respiratory syncytial virus (RSV) A in 13 of 15 (86.7%) positive control samples. Additionally, rotavirus, torque teno virus, human papillomavirus, human betaherpesvirus 7, cyclovirus, vientovirus, gemycircularvirus, and statovirus were identified through mNGS. Notably, complete genomes of novel cyclovirus, gemycircularvirus, and statovirus were genetically characterized. Using PCR screening, the novel cyclovirus was additionally detected in 5 and the novel gemycircularvirus in 12 of the remaining samples included for mNGS analysis. Our studies therefore provide pioneering data of the virome of acute-respiratory diseases from individuals at risk of zoonotic infections. The mNGS protocol/pipeline applied here is sensitive for the detection of a variety of viruses, including novel ones. More frequent detections of the novel viruses by PCR than by mNGS on the same samples suggests that PCR remains the most sensitive. � 2020 by the authors.

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