AUTHOR=Duah-Quashie Nancy Odurowah , Opoku-Agyeman Philip , Bruku Selassie , Adams Tryphena , Tandoh Kwesi Zandoh , Ennuson Nana Aba , Matrevi Sena Adzoa , Abuaku Benjamin , Quashie Neils Ben , Watters Chaselynn , Wolfe David , Quijada Hugo Miranda , Sanders Terrel 

TITLE=Genetic deletions and high diversity of Plasmodium falciparum histidine-rich proteins 2 and 3 genes in parasite populations in Ghana

JOURNAL=Frontiers in Epidemiology

VOLUME=2

YEAR=2022

URL=https://www.frontiersin.org/journals/epidemiology/articles/10.3389/fepid.2022.1011938

DOI=10.3389/fepid.2022.1011938

ISSN=2674-1199

ABSTRACT=<p>Rapid diagnostic tests (RDTs) are used to diagnose malaria in Ghana and other malaria endemic countries. <italic>Plasmodium falciparum</italic> histidine-rich protein 2 (PFHRP2<italic>)</italic> based RDTs are widely used, however the occurrence of deletions of the <italic>pfhrp2</italic> gene in some parasites have resulted in false negative test results. Monoclonal antibodies of PFHRP2 cross reacts with PFHRP3 because they share structural similarities and this complements the detection of the parasites by RDT. These two genes were investigated in Ghanaian <italic>P. falciparum</italic> parasite population to detect deletions and the polymorphisms in exon 2 of the <italic>pfhrp2</italic> and <italic>pfhrp3</italic> genes. Parasite isolates (2,540) from children ≤ 12 years with uncomplicated malaria from 2015 to 2020 transmission seasons were used. Both genes were amplified using nested PCR and negative results indicated the presence of the deletion of genes. Amplified genes were sequenced for the detection of the amino acid repeats. Deletions were observed in 30.7% (780/2,540) and 17.2% (438/2,540) of the samples for <italic>pfhrp2</italic> and <italic>pfhrp3</italic> respectively with increasing trends over the three time periods (χ2 −10.305, <italic>p</italic> = 0.001). A total of 1,632 amplicons were sequenced for each gene, analysis was done on 1,124 and 1,307 good quality sequences for <italic>pfhrp2</italic> and <italic>pfhrp3</italic> respectively. <italic>Pfhrp2</italic> repeat polymorphisms were dominantly of types 2 (AHHAHHAAD) and 7 (AHHAAD) with large numbers of variants. A novel variant of type 14 (AHHANHATD) was seen for <italic>pfhrp2</italic>. For the <italic>pfhrp3</italic> repeat types, 16 (AHHAAN), 17 (AHHDG) and 18 (AHHDD) were the dominant types observed. Variants of type 16 (AHHAAH) and (AHHASH) were also dominant. Repeat types 1, 2, 3, 4, 5, 6, 7, 8, 11, 13, 15, 16, and 19 were observed be shared by both genes. The haplotype diversity of both genes ranged between 0.872 and 1 indicating high diversity of the polymorphisms in the isolates. The implication of the findings of the frequencies of the <italic>pfhrp2</italic> and <italic>pfhrp3</italic> deletions as well as the variants of the main epitopes of the monoclonal antibodies for the RDT (types 2 and 7) in our isolates is an indication of decreased sensitivity of the RDTs in diagnosing malaria infections in Ghana.</p>