Nanopore sequencing for real-time genomic surveillance ofPlasmodium falciparum

Author:

Girgis Sophia T.,Adika Edem,Nenyewodey Felix E.,Senoo Jnr Dodzi K.,Ngoi Joyce M.,Bandoh Kukua,Lorenz Oliver,van de Steeg Guus,Nsoh Sebastian,Judge Kim,Pearson Richard D.,Almagro-Garcia Jacob,Saiid Samirah,Atampah Solomon,Amoako Enock K.,Morang’a Collins M.,Asoala Victor,Adjei Elrmion S.,Burden William,Roberts-Sengier William,Drury Eleanor,Gonçalves Sónia,Awandare Gordon A.,Kwiatkowski Dominic P.,Amenga-Etego Lucas N.,Hamilton William L.ORCID

Abstract

AbstractMalaria is a global public health priority causing over 600,000 deaths annually, mostly young children living in Sub-Saharan Africa. Molecular surveillance can provide key information for malaria control, such as the prevalence and distribution of antimalarial drug resistance. However, genome sequencing capacity in endemic countries can be limited. Here, we have implemented an end-to-end workflow forP. falciparumgenomic surveillance in Ghana using Oxford Nanopore Technologies, targeting antimalarial resistance markers and the leading vaccine antigencircumsporozoite protein(csp). The workflow was rapid, robust, accurate, affordable and straightforward to implement. We found thatP. falciparumparasites in Ghana had become largely susceptible to chloroquine, with persistent sulfadoxine-pyrimethamine (SP) resistance, and no evidence of artemisinin resistance. Multiple Single Nucleotide Polymorphism (SNP) differences from the vaccinecspsequence were identified, though their significance is uncertain. This study demonstrates the potential utility and feasibility of malaria genomic surveillance in endemic settings using Nanopore sequencing.

Publisher

Cold Spring Harbor Laboratory

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