Comparison of molecular surveillance methods to assess changes in the population genetics of Plasmodium falciparum in high transmission

Anita Ghansah; Kathryn E. Tiedje; Dionne C. Argyropoulos; Christiana O. Onwona; Samantha L. Deed; Frédéric Labbé; Abraham R. Oduro; Kwadwo A. Koram; Mercedes Pascual; Karen P. Day

doi:10.3389/fpara.2023.1067966

Comparison of molecular surveillance methods to assess changes in the population genetics of Plasmodium falciparum in high transmission

Anita Ghansah, Kathryn E. Tiedje, Dionne C. Argyropoulos, Christiana O. Onwona, Samantha L. Deed, Frédéric Labbé, Abraham R. Oduro, Kwadwo A. Koram, Mercedes Pascual, Karen P. Day

Biology and Genomics

Research output: Contribution to journal › Article › peer-review

Abstract

A major motivation for developing molecular methods for malaria surveillance is to measure the impact of control interventions on the population genetics of Plasmodium falciparum as a potential marker of progress towards elimination. Here we assess three established methods (i) single nucleotide polymorphism (SNP) barcoding (panel of 24-biallelic loci), (ii) microsatellite genotyping (panel of 12-multiallelic loci), and (iii) varcoding (fingerprinting var gene diversity, akin to microhaplotyping) to identify changes in parasite population genetics in response to a short-term indoor residual spraying (IRS) intervention. Typical of high seasonal transmission in Africa, multiclonal infections were found in 82.3% (median 3; range 1-18) and 57.8% (median 2; range 1-12) of asymptomatic individuals pre- and post-IRS, respectively, in Bongo District, Ghana. Since directly phasing multilocus haplotypes for population genetic analysis is not possible for biallelic SNPs and microsatellites, we chose ~200 low-complexity infections biased to single and double clone infections for analysis. Each genotyping method presented a different pattern of change in diversity and population structure as a consequence of variability in usable data and the relative polymorphism of the molecular markers (i.e., SNPs < microsatellites < var). Varcoding and microsatellite genotyping showed the overall failure of the IRS intervention to significantly change the population structure from pre-IRS characteristics (i.e., many diverse genomes of low genetic similarity). The 24-SNP barcode provided limited information for analysis, largely due to the biallelic nature of SNPs leading to a high proportion of double-allele calls and a view of more isolate relatedness compared to microsatellites and varcoding. Relative performance, suitability, and cost-effectiveness of the methods relevant to sample size and local malaria elimination in high-transmission endemic areas are discussed.

Original language	English (US)
Article number	1067966
Journal	Frontiers in Parasitology
Volume	2
DOIs	https://doi.org/10.3389/fpara.2023.1067966
State	Published - 2023

Keywords

high transmission
malaria control interventions
microsatellies
molecular markers
Plasmodium falciparum
population genetics
SNPs (single nucleotide polymorphisms)
var genes

ASJC Scopus subject areas

Parasitology
Infectious Diseases
veterinary (miscalleneous)

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10.3389/fpara.2023.1067966

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Ghansah, A., Tiedje, K. E., Argyropoulos, D. C., Onwona, C. O., Deed, S. L., Labbé, F., Oduro, A. R., Koram, K. A., Pascual, M., & Day, K. P. (2023). Comparison of molecular surveillance methods to assess changes in the population genetics of Plasmodium falciparum in high transmission. Frontiers in Parasitology, 2, Article 1067966. https://doi.org/10.3389/fpara.2023.1067966

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abstract = "A major motivation for developing molecular methods for malaria surveillance is to measure the impact of control interventions on the population genetics of Plasmodium falciparum as a potential marker of progress towards elimination. Here we assess three established methods (i) single nucleotide polymorphism (SNP) barcoding (panel of 24-biallelic loci), (ii) microsatellite genotyping (panel of 12-multiallelic loci), and (iii) varcoding (fingerprinting var gene diversity, akin to microhaplotyping) to identify changes in parasite population genetics in response to a short-term indoor residual spraying (IRS) intervention. Typical of high seasonal transmission in Africa, multiclonal infections were found in 82.3% (median 3; range 1-18) and 57.8% (median 2; range 1-12) of asymptomatic individuals pre- and post-IRS, respectively, in Bongo District, Ghana. Since directly phasing multilocus haplotypes for population genetic analysis is not possible for biallelic SNPs and microsatellites, we chose ~200 low-complexity infections biased to single and double clone infections for analysis. Each genotyping method presented a different pattern of change in diversity and population structure as a consequence of variability in usable data and the relative polymorphism of the molecular markers (i.e., SNPs < microsatellites < var). Varcoding and microsatellite genotyping showed the overall failure of the IRS intervention to significantly change the population structure from pre-IRS characteristics (i.e., many diverse genomes of low genetic similarity). The 24-SNP barcode provided limited information for analysis, largely due to the biallelic nature of SNPs leading to a high proportion of double-allele calls and a view of more isolate relatedness compared to microsatellites and varcoding. Relative performance, suitability, and cost-effectiveness of the methods relevant to sample size and local malaria elimination in high-transmission endemic areas are discussed.",

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AU - Ghansah, Anita

AU - Tiedje, Kathryn E.

AU - Argyropoulos, Dionne C.

AU - Onwona, Christiana O.

AU - Deed, Samantha L.

AU - Labbé, Frédéric

AU - Oduro, Abraham R.

AU - Koram, Kwadwo A.

AU - Pascual, Mercedes

AU - Day, Karen P.

PY - 2023

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AB - A major motivation for developing molecular methods for malaria surveillance is to measure the impact of control interventions on the population genetics of Plasmodium falciparum as a potential marker of progress towards elimination. Here we assess three established methods (i) single nucleotide polymorphism (SNP) barcoding (panel of 24-biallelic loci), (ii) microsatellite genotyping (panel of 12-multiallelic loci), and (iii) varcoding (fingerprinting var gene diversity, akin to microhaplotyping) to identify changes in parasite population genetics in response to a short-term indoor residual spraying (IRS) intervention. Typical of high seasonal transmission in Africa, multiclonal infections were found in 82.3% (median 3; range 1-18) and 57.8% (median 2; range 1-12) of asymptomatic individuals pre- and post-IRS, respectively, in Bongo District, Ghana. Since directly phasing multilocus haplotypes for population genetic analysis is not possible for biallelic SNPs and microsatellites, we chose ~200 low-complexity infections biased to single and double clone infections for analysis. Each genotyping method presented a different pattern of change in diversity and population structure as a consequence of variability in usable data and the relative polymorphism of the molecular markers (i.e., SNPs < microsatellites < var). Varcoding and microsatellite genotyping showed the overall failure of the IRS intervention to significantly change the population structure from pre-IRS characteristics (i.e., many diverse genomes of low genetic similarity). The 24-SNP barcode provided limited information for analysis, largely due to the biallelic nature of SNPs leading to a high proportion of double-allele calls and a view of more isolate relatedness compared to microsatellites and varcoding. Relative performance, suitability, and cost-effectiveness of the methods relevant to sample size and local malaria elimination in high-transmission endemic areas are discussed.

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Comparison of molecular surveillance methods to assess changes in the population genetics of Plasmodium falciparum in high transmission

Abstract

Keywords

ASJC Scopus subject areas

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