Genotyping Plasmodium falciparum gametocytes using amplicon deep sequencing

Jimmy Vareta; Natalie A Horstman; Matthew Adams; Karl B Seydel; Robert S McCann; Lauren M Cohee; Miriam K Laufer; Shannon Takala-Harrison

doi:10.1186/s12936-024-04920-3

Genotyping Plasmodium falciparum gametocytes using amplicon deep sequencing

Malar J. 2024 Apr 6;23(1):96. doi: 10.1186/s12936-024-04920-3.

Authors

Jimmy Vareta¹, Natalie A Horstman^{1

2}, Matthew Adams¹, Karl B Seydel^{3

4}, Robert S McCann¹, Lauren M Cohee¹, Miriam K Laufer¹, Shannon Takala-Harrison⁵

Affiliations

¹ Center for Vaccine Development and Global Health, University of Maryland School of Medicine, Baltimore, MD, USA.
² Division of Cardiology, Department of Medicine, Johns Hopkins University School of Medicine, Baltimore, MD, USA.
³ Blantyre Malaria Project, Kamuzu University of Health Sciences, Blantyre, Malawi.
⁴ College of Osteopathic Medicine, Michigan State University, East Lansing, MI, USA.
⁵ Center for Vaccine Development and Global Health, University of Maryland School of Medicine, Baltimore, MD, USA. stakala@som.umaryland.edu.

Abstract

Background: Understanding the dynamics of gametocyte production in polyclonal Plasmodium falciparum infections requires a genotyping method that detects distinct gametocyte clones and estimates their relative frequencies. Here, a marker was identified and evaluated to genotype P. falciparum mature gametocytes using amplicon deep sequencing.

Methods: A data set of polymorphic regions of the P. falciparum genome was mined to identify a gametocyte genotyping marker. To assess marker resolution, the number of unique haplotypes in the marker region was estimated from 95 Malawian P. falciparum whole genome sequences. Specificity of the marker for detection of mature gametocytes was evaluated using reverse transcription-polymerase chain reaction of RNA extracted from NF54 mature gametocytes and rings from a non-gametocyte-producing strain of P. falciparum. Amplicon deep sequencing was performed on experimental mixtures of mature gametocytes from two distinct parasite clones, as well as gametocyte-positive P. falciparum field isolates to evaluate the quantitative ability and determine the limit of detection of the genotyping approach.

Results: A 400 bp region of the pfs230 gene was identified as a gametocyte genotyping marker. A larger number of unique haplotypes was observed at the pfs230 marker (34) compared to the sera-2 (18) and ama-1 (14) markers in field isolates from Malawi. RNA and DNA genotyping accurately estimated gametocyte and total parasite clone frequencies when evaluating agreement between expected and observed haplotype frequencies in gametocyte mixtures, with concordance correlation coefficients of 0.97 [95% CI: 0.92-0.99] and 0.92 [95% CI: 0.83-0.97], respectively. The detection limit of the genotyping method for male gametocytes was 0.41 pfmget transcripts/µl [95% CI: 0.28-0.72] and for female gametocytes was 1.98 ccp4 transcripts/µl [95% CI: 1.35-3.68].

Conclusions: A region of the pfs230 gene was identified as a marker to genotype P. falciparum gametocytes. Amplicon deep sequencing of this marker can be used to estimate the number and relative frequency of parasite clones among mature gametocytes within P. falciparum infections. This gametocyte genotyping marker will be an important tool for studies aimed at understanding dynamics of gametocyte production in polyclonal P. falciparum infections.

Keywords: Plasmodium falciparum; Amplicon deep sequencing; Complexity of infection; Gametocyte genotyping; Malaria transmission.

MeSH terms

Female
Genotype
High-Throughput Nucleotide Sequencing
Humans
Malaria, Falciparum* / parasitology
Male
Plasmodium falciparum* / genetics
RNA

Substances

RNA

Abstract

MeSH terms

Substances

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