Fine-scale genomic tracking of Ross River virus using nanopore sequencing

Ellen M de Vries; Noel O I Cogan; Aneta J Gubala; Brendan C Rodoni; Stacey E Lynch

doi:10.1186/s13071-023-05734-z

Fine-scale genomic tracking of Ross River virus using nanopore sequencing

Parasit Vectors. 2023 Jun 6;16(1):186. doi: 10.1186/s13071-023-05734-z.

Authors

Ellen M de Vries^{1

2}, Noel O I Cogan^{3

4}, Aneta J Gubala⁵, Brendan C Rodoni^{3

4}, Stacey E Lynch³

Affiliations

¹ Agriculture Victoria, AgriBio, Centre for AgriBioscience, Bundoora, VIC, 3083, Australia. ellen.devries@agriculture.vic.gov.au.
² School of Applied Systems Biology, La Trobe University, Bundoora, VIC, 3083, Australia. ellen.devries@agriculture.vic.gov.au.
³ Agriculture Victoria, AgriBio, Centre for AgriBioscience, Bundoora, VIC, 3083, Australia.
⁴ School of Applied Systems Biology, La Trobe University, Bundoora, VIC, 3083, Australia.
⁵ Sensors and Effectors Division, Defence Science & Technology Group, Fishermans Bend, VIC, 3207, Australia.

Abstract

Background: Ross River virus (RRV) is Australia's most common and widespread mosquito-transmitted arbovirus and is of significant public health concern. With increasing anthropogenic impacts on wildlife and mosquito populations, it is important that we understand how RRV circulates in its endemic hotspots to determine where public health efforts should be directed. Current surveillance methods are effective in locating the virus but do not provide data on the circulation of the virus and its strains within the environment. This study examined the ability to identify single nucleotide polymorphisms (SNPs) within the variable E2/E3 region by generating full-length haplotypes from a range of mosquito trap-derived samples.

Methods: A novel tiled primer amplification workflow for amplifying RRV was developed with analysis using Oxford Nanopore Technology's MinION and a custom ARTIC/InterARTIC bioinformatic protocol. By creating a range of amplicons across the whole genome, fine-scale SNP analysis was enabled by specifically targeting the variable region that was amplified as a single fragment and established haplotypes that informed spatial-temporal variation of RRV in the study site in Victoria.

Results: A bioinformatic and laboratory pipeline was successfully designed and implemented on mosquito whole trap homogenates. Resulting data showed that genotyping could be conducted in real time and that whole trap consensus of the viruses (with major SNPs) could be determined in a timely manner. Minor variants were successfully detected from the variable E2/E3 region of RRV, which allowed haplotype determination within complex mosquito homogenate samples.

Conclusions: The novel bioinformatic and wet laboratory methods developed here will enable fast detection and characterisation of RRV isolates. The concepts presented in this body of work are transferable to other viruses that exist as quasispecies in samples. The ability to detect minor SNPs, and thus haplotype strains, is critically important for understanding the epidemiology of viruses their natural environment.

Keywords: Bioinformatics; Nanopore; Ross River virus; SNP analysis; Tiled amplicon sequencing.

MeSH terms

Alphavirus Infections*
Animals
Culicidae*
Genomics
Humans
Nanopore Sequencing*
Ross River virus / genetics

Grants and funding

G12017SRodoniLaT459/Defence Science Institute