4.7 Article

High-throughput barcoding method for the genetic surveillance of insecticide resistance and species identification in Anopheles gambiae complex malaria vectors

Journal

SCIENTIFIC REPORTS
Volume 12, Issue 1, Pages -

Publisher

NATURE PORTFOLIO
DOI: 10.1038/s41598-022-17822-8

Keywords

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Funding

  1. Newton Institutional Links Grant (British Council) [261868591]
  2. Medical Research Council UK [MR/M01360X/1, MR/R025576/1, MR/R020973/1, MR/N010469/1]
  3. BBSRC [BB/R013063/1]
  4. MRC LiD Ph.D. studentship
  5. Nagasaki University Doctoral Program for World-leading Innovative and Smart Education for Global Health (Ministry of Education, Culture, Sports, Science, and Technology of Japan)
  6. Foreign, Commonwealth & Development Office (FCDO)
  7. Wellcome
  8. Department of Health and Social Care [MR/R006040/1]
  9. Foreign, Commonwealth & Development Office (FCDO) RPC
  10. Wellcome Trust Biomedical Resources grant
  11. Wellcome Trust/Royal Society Sir Henry Dale Fellowship [101285/Z/13/Z]
  12. [R01AI123074]

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Surveillance of malaria vector species and monitoring of insecticide resistance are crucial for informing malaria control strategies. This study developed a high-throughput panel using genetic barcoding, PCR, and next-generation sequencing to monitor Anopheles mosquitoes in malaria endemic regions. The panel successfully detected Plasmodium infection and insecticide resistance mutations in four Anapheles species, providing a reliable and cost-effective approach for surveillance.
Surveillance of malaria vector species and the monitoring of insecticide resistance are essential to inform malaria control strategies and support the reduction of infections and disease. Genetic barcoding of mosquitoes is a useful tool to assist the high-throughput surveillance of insecticide resistance, discriminate between sibling species and to detect the presence of Plasmodium infections. In this study, we combined multiplex PCR, custom designed dual indexing, and Illumina next generation sequencing for high throughput single nucleotide polymorphism (SNP)-profiling of four species from the Anopheles (An.) gambiae complex (An. gambiae sensu stricto, An. coluzzii, An. arabiensis and An. melas). By amplifying and sequencing only 14 genetic fragments (500 bp each), we were able to simultaneously detect Plasmodium infection; insecticide resistance-conferring SNPs in ace1, gste2, vgsc and rdl genes; the partial sequences of nuclear ribosomal internal transcribed spacers (ITS1 and ITS2) and intergenic spacers (IGS), Short INterspersed Elements (SINE), as well as mitochondrial genes (cox1 and nd4) for species identification and genetic diversity. Using this amplicon sequencing approach with the four selected An. gambiae complex species, we identified a total of 15 non-synonymous mutations in the insecticide target genes, including previously described mutations associated with resistance and two new mutations (F1525L in vgsc and D148E in gste2). Overall, we present a reliable and cost-effective high-throughput panel for surveillance of An. gambiae complex mosquitoes in malaria endemic regions.

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