Affiliation:
1. London School of Hygiene & Tropical Medicine
2. Armauer Hansen Research Institute
3. Radboud University Nijmegen Medical Centre
4. University of Nevada, Las Vegas
Abstract
Abstract
Since its first detection in 2012 in Djibouti, Anopheles stephensi has invaded and established itself in the Horn of Africa and most recently in Nigeria and Yemen. The expansion of this vector poses a significant threat to malaria control and eliminations efforts. Integrated vector management is the primary strategy used to interrupt disease transmission; however, growing insecticide resistance is threatening to reverse gains in global malaria control. We present a next-generation amplicon-sequencing approach, for high-throughput monitoring of insecticide resistance genes (ace1, gste2, vgsc and rdl), species identification and characterization of genetic diversity (its2 and cox1) in An. stephensi. Ninety-five An. stephensi mosquitoes, collected in Ethiopia, were screened, identifying 104 SNPs, including the knock-down mutation L958F (L1014F in Musca domestica), and for the first time in this vector species, the A296S substitution (A301S in Drosophila melanogaster) in the rdl locus. Two other amino acid substitutions (ace1-N177D, GSTe2-V189L) were also identified but have not been previously implicated in insecticide resistance. Genetic diversity in the mitochondrial cox1 gene revealed shared haplotypes between Ethiopian An. stephensi with samples from Pakistan, Sudan, and Djibouti. Overall, we present a reliable, cost-effective strategy using amplicon-sequencing to monitor known insecticide resistance mutations, with the potential to identify new genetic variants, to assist high-throughput surveillance of An. stephensi populations.
Publisher
Research Square Platform LLC
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