Rapid molecular assays for the detection of the four dengue viruses in infected mosquitoes [version 2; peer review: 2 approved]

Joanne Macdonald; Madeeha Ahmed; Leon E. Hugo; Nina M. Pollak; Jody Hobson-Peters; Andrew F. van den Hurk

Gates Open Research (Dec 2022)

Rapid molecular assays for the detection of the four dengue viruses in infected mosquitoes [version 2; peer review: 2 approved]

Joanne Macdonald,
Madeeha Ahmed,
Leon E. Hugo,
Nina M. Pollak,
Jody Hobson-Peters,
Andrew F. van den Hurk

Affiliations

Joanne Macdonald: ORCiD; Centre for Bioinnovation, University of the Sunshine Coast, Sippy Downs, QLD, 4556, Australia
Madeeha Ahmed: ORCiD; Centre for Bioinnovation, University of the Sunshine Coast, Sippy Downs, QLD, 4556, Australia
Leon E. Hugo: Mosquito Control Laboratory, QIMR Berghofer Medical Research Institute, Herston, QLD, 4006, Australia
Nina M. Pollak: Centre for Bioinnovation, University of the Sunshine Coast, Sippy Downs, QLD, 4556, Australia
Jody Hobson-Peters: Australian Infectious Diseases Research Centre, School of Chemistry and Molecular Biosciences, The University of Queensland, St Lucia, QLD, 4072, Australia
Andrew F. van den Hurk: Public Health Virology, Forensic and Scientific Services, Department of Health, Queensland Government, Coopers Plains, QLD, 4108, Australia

Journal volume & issue: Vol. 6

Abstract

Read online

The pantropic emergence of severe dengue disease can partly be attributed to the co-circulation of different dengue viruses (DENVs) in the same geographical location. Effective monitoring for circulation of each of the four DENVs is critical to inform disease mitigation strategies. In low resource settings, this can be effectively achieved by utilizing inexpensive, rapid, sensitive and specific assays to detect viruses in mosquito populations. In this study, we developed four rapid DENV tests with direct applicability for low-resource virus surveillance in mosquitoes. The test protocols utilize a novel sample preparation step, a single-temperature isothermal amplification, and a simple lateral flow detection. Analytical sensitivity testing demonstrated tests could detect down to 1,000 copies/µL of virus-specific DENV RNA, and analytical specificity testing indicated tests were highly specific for their respective virus, and did not detect closely related flaviviruses. All four DENV tests showed excellent diagnostic specificity and sensitivity when used for detection of both individually infected mosquitoes and infected mosquitoes in pools of uninfected mosquitoes. With individually infected mosquitoes, the rapid DENV-1, -2 and -3 tests showed 100% diagnostic sensitivity (95% CI = 69% to 100%, n=8 for DENV-1; n=10 for DENV 2,3) and the DENV-4 test showed 92% diagnostic sensitivity (CI: 62% to 100%, n=12) along with 100% diagnostic specificity (CI: 48–100%) for all four tests. Testing infected mosquito pools, the rapid DENV-2, -3 and -4 tests showed 100% diagnostic sensitivity (95% CI = 69% to 100%, n=10) and the DENV-1 test showed 90% diagnostic sensitivity (55.50% to 99.75%, n=10) together with 100% diagnostic specificity (CI: 48–100%). Our tests reduce the operational time required to perform mosquito infection status surveillance testing from > two hours to only 35 minutes, and have potential to improve accessibility of mosquito screening, improving monitoring and control strategies in low-income countries most affected by dengue outbreaks.

Published in Gates Open Research

ISSN: 2572-4754 (Online)
Publisher: F1000 Research Ltd
Country of publisher: United Kingdom
LCC subjects: Medicine
Website: https://gatesopenresearch.org/

About the journal

Abstract

Keywords