Novel multiplex family-wide PCR and Nanopore sequencing of amplicons (FP-NSA) approach for surveillance of influenza- and coronaviruses in humans and animals
Title (eng)
Novel multiplex family-wide PCR and Nanopore sequencing of amplicons (FP-NSA) approach for surveillance of influenza- and coronaviruses in humans and animals
Author
Irene Kasindi Meki
Ki Bum Ahn
William G. Dundon
Tirumala Bharani K. Settypalli
Christoph Leth
Adi Steinrigl
Sandra Revilla-Fernández
Friedrich Schmoll
Letizia Ceglie
Kouramoudou Berete
Artem Metlin
Madhur Dhingra
Giovanni Cattoli
Charles Euloge Lamien
Abstract (eng)
Background
Recent outbreaks of zoonotic diseases like Ebola, Mpox, dengue fever, and COVID-19 highlight gaps in surveillance and early detection at disease hotspots. Virus family-wide diagnostic assays offer a cost-effective and sensitive alternative to metagenomics for initial virus identification. This study introduces a multiplex family-wide PCR coupled with Nanopore sequencing of amplicons (FP-NSA) for surveillance of novel and known zoonotic respiratory viruses, including influenza A and D viruses (IAV and IDV), alpha (α-), beta (β-), and gamma (γ-) coronaviruses (CoVs).
Methods
This assay utilized primers in conserved regions of each virus group for multiplex reverse transcription (RT)-PCR coupled with the portable MinION device for rapid Nanopore sequencing. The FP-NSA was optimized using seven IAV subtypes, IDVs, and α- and β-CoVs. The analytical sensitivity of the FP-NSA was assessed using positive controls of known concentrations from each targeted viral family and validated using clinical samples and cell culture isolates from various host species and geographical origins. Potential novel viruses detected in the clinical samples, based on the FP-NSA, were further analyzed using metagenomics sequencing with the Sequence-Independent Single Primer Amplification (SISPA) approach.
Results
The optimized FP-NSA assay efficiently detected all the targeted viruses singly as well as in co-infection scenarios of multiple respiratory viruses. Evaluation of the assay on 78 selected clinical and cell culture samples (from 184 initially screened) successfully detected IAVs; α-CoVs: porcine epidemic diarrhea virus (PEDV), human coronavirus (HCoV) NL63, and HCoV-229E; β-CoVs: HCoV-OC43, severe acute respiratory syndrome (SARS)-CoV-(1), SARS-CoV-2, and MERS-CoV; and γ-CoV infectious bronchitis virus (γ-CoV_IBV) infections. Additionally, the FP-NSA assay discovered a novel γ-CoV_IBV from Guinea that is phylogenetically distant from known genotypes using a SISPA metagenomics approach.
Conclusions
The assay’s short PCR amplicons enable screening of samples within 4 h, from PCR to sequencing and bioinformatics analysis, providing an adequate number of pathogens’ reads. The portable MinION device makes the assay suitable for pathogen surveillance in disease hotspots and resource-limited regions such as low- and middle-income countries. Thus, the FP-NSA assay is a valuable tool for detecting potential novel and known zoonotic respiratory viruses in the targeted families across various host species.
Keywords (eng)
Zoonotic Respiratory VirusesFP-NSANanopore SequencingMultiplex RT-PCRSurveillance
Type (eng)
Language
[eng]
Persistent identifier
Is in series
Title (eng)
Genome Medicine
Volume
17
Issue
1
ISSN
1756-994X
Issued
2025
Number of pages
14
Publication
Springer
Version type (eng)
Date issued
2025
Access rights (eng)
License
Rights statement (eng)
© 2025, The Author(s)
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https://phaidra.vetmeduni.ac.at/o:5119 - Other links and identifiers
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- RightsLicenseRights statement© 2025, The Author(s)
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