Abstract

Population genetic analysis of Plasmodium falciparum parasites using a customized Illumina GoldenGate genotyping assay

Campino S, Auburn S, Kivinen K, Zongo I, Ouedraogo JB, Mangano V, Djimde A, Doumbo OK, Kiara SM, Nzila A, Borrmann S, Marsh K, Michon P, Mueller I, Siba P, Jiang H, Su XZ, Amaratunga C, Socheat D, Fairhurst RM, Imwong M, Anderson T, Nosten F, White NJ, Gwilliam R, Deloukas P, MacInnis B, Newbold CI, Rockett K, Clark TG, Kwiatkowski DP
PLoS One. 2011;6

Permenent descriptor
https://doi.org/10.1371/journal.pone.0020251


The diversity in the Plasmodium falciparum genome can be used to explore parasite population dynamics, with practical applications to malaria control. The ability to identify the geographic origin and trace the migratory patterns of parasites with clinically important phenotypes such as drug resistance is particularly relevant. With increasing single-nucleotide polymorphism (SNP) discovery from ongoing Plasmodium genome sequencing projects, a demand for high SNP and sample throughput genotyping platforms for large-scale population genetic studies is required. Low parasitaemias and multiple clone infections present a number of challenges to genotyping P. falciparum. We addressed some of these issues using a custom 384-SNP Illumina GoldenGate assay on P. falciparum DNA from laboratory clones (long-term cultured adapted parasite clones), short-term cultured parasite isolates and clinical (non-cultured isolates) samples from East and West Africa, Southeast Asia and Oceania. Eighty percent of the SNPs (n = 306) produced reliable genotype calls on samples containing as little as 2 ng of total genomic DNA and on whole genome amplified DNA. Analysis of artificial mixtures of laboratory clones demonstrated high genotype calling specificity and moderate sensitivity to call minor frequency alleles. Clear resolution of geographically distinct populations was demonstrated using Principal Components Analysis (PCA), and global patterns of population genetic diversity were consistent with previous reports. These results validate the utility of the platform in performing population genetic studies of P. falciparum.

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Key Terms
Cloning, Organism | Culture Techniques | DNA, Protozoan/genetics/isolation & purification | Genetic Loci/genetics | Genotype | High-Throughput Nucleotide Sequencing/ methods | Laboratories | Malaria, Falciparum | Plasmodium falciparum/ genetics/growth & development/ isolation & | purification/physiology (Source: Medline)
Funded by
Bill and Melinda Gates Foundation; Wellcome Trust; Medical Research Council-UK; European Developing Countries Clinical Trials Partnership; Division of Intramural Research of the National Institutes of Health and National Institute of Allergy and Infectious Diseases-USA; National Health and Medical Research Council-Australia; National Malaria Control Program; National Budget of the Institut de Recherche en Sciences de le Sante-Burkina Faso; Howard Hughes Medical Institution International Scholarship; Medical Research Council [G19/9, G0600718] Funding Source: researchfish; MRC [G0600718, G19/9] Funding Source: UKRI; NATIONAL INSTITUTE OF ALLERGY AND INFECTIOUS DISEASES [ZIAAI001066, ZIAAI001000, R37AI048071] Funding Source: NIH RePORTER
External Sources
Abstract at pubmed
Full text at publishers website
Full text at PMC