Large-scale survey for novel genotypes of Plasmodium falciparum chloroquine-resistance gene pfcrt

Blood samples were obtained from P. falciparum-infected individuals living in eight malaria endemic countries as follows.

Before enrolment, written informed consent was obtained from all study subjects. In the case of children, consent was obtained from a parent or legal guardian. This study was approved by (1) The Institutional Ethics Committee of the Thai Ministry of Public Health, the Human Subjects Research Review Board of the United States Army, (2) The Center of Malariology, Parasitology and Entomology (CMPE), Lao P.D.R., the Research Committee of the Ministry of Public Health (MoPH), Lao P.D.R., (3) The National Center for Parasitology, Entomology and Malaria Control (CNM), Cambodia, (4) The Bangladesh Medical Research Council and the local regulatory body of health in Bandarban, Bangladesh, (5) The Palawan Provincial Health Office, Philippines, (6) The National Department of Health Medical Research Advisory Committee of Papua New Guinea, (7) The Vanuatu Department of Health, Vanuatu, and (8) The Ministry of Health/Ghana Health Service, Ghana.

Finger-prick blood was spotted onto chromatography filter paper ET31CHR (Whatman, Maidstone, UK) in Lao P.D.R., Cambodia, Bangladesh, Papua New Guinea, Vanuatu and Ghana. In Thailand and the Philippines, venous blood was transferred into heparin-containing test tubes. Parasite DNA was extracted using QIAamp DNA mini kits (Qiagen, Hilden, Germany) from a quarter of a dried blood spot or a corresponding amount of blood (25 μl), in accordance with the manufacturer's instructions. The Lao P.D.R. and Bangladesh samples were extracted using QIAamp DNA mini kits with the QIAcube™ (Qiagen) tissue protocol.

The pfcrt gene was amplified by nested PCR using two sets of primers designed to amplify a region of exon 2 including known polymorphic sites at amino acid positions 72, 74, 75 and 76. PCR primers were designed after the sequence of 3D7 clone [GenBank: NC_004328]. Primer sequences and PCR conditions are shown in Additional file 1. Amplified product (aa 57-120) was purified using ExoSAP-IT (GE Healthcare UK Ltd., Buckinghamshire, UK) and were directly sequenced with a DYEnamic ET terminator kit in the MegaBACE 1000 DNA sequencer (GE Healthcare UK Ltd.). Data on pfcrt genotypes previously obtained from Papua New Guinea were included in the present analysis [32].

Variations in the number of TA repeats located at 0.59 kb, 10.389 kb, 23.576 kb, -2.814 kb and -29.268 kb in pfcrt and ATT repeats located at 10.389 kb in pfcrt were measured using PCR protocol previously described with some modifications (Additional file 2) [34]. Briefly, each MS marker was amplified by semi-nested PCR using fluorescent 5'-end labeled primers (Applied Biosystems., Foster city, CA, USA) in an ABI 2720 thermal cycler (Applied Biosystems). Amplified products were analysed using an ABI 377 DNA sequencer and GeneScan 3.1.2 software with GENESCAN™ 400 HD ROX size standard (Applied Biosystems), followed by size determination using a Genotyper 2.0 (Applied Biosystems). When two or more polymorphisms were detected, these isolates were considered to be mixed infections and excluded them from further analysis. As it has been well documented that wild-type parasites show extensive MS variations due to the lack of selective CQ sweeps [1], MS haplotypes were determined only for pfcrt mutant isolates.

In order to assess the genetic relationships among CQ-resistant pfcrt genotypes, a median-joining haplotype network was constructed based on alleles at the six MS loci using the Network 4.6 software [35]. Median joining is a method for constructing genetic networks to identify the minimum spanning tree by favouring short connections [35].

Among 263 P. falciparum isolates examined in this study, pfcrt genotypes were successfully determined in 256 samples. In addition to the wild-type CVMNK (10%), four pfcrt mutant genotypes were identified; CVIET (48%), CVIDT (6%), S VMNT (33%) and CVMNT (1%). Mixed genotypes were observed in four samples (2%) (Figure 1). In endemic regions of Indochina (Thai and Cambodia), South Asia (Bangladesh) and Africa (Ghana), CVIET was the predominant mutant genotype, which is consistent with previous studies [1, 11]. One exception was Lao P.D.R., where the wild genotype and CVIDT were equally predominant, with CVIET showing a low frequency. In the Philippines, as previously observed [14], S VMNT was the dominant mutant genotype, and CVMNT was also found. In Melanesia, only S VMNT was found as a mutant genotype, as reported previously [36]. We did not observe any novel mutations at amino acid positions 57-120, other than those known at positions 72, 74, 75 and 76.

Among 227 isolates harbouring pfcrt mutant genotypes, 196 samples were successfully determined for MS haplotypes. In total, 49 MS haplotypes were identified, including the three previously known major haplotypes (IC1, M1 and P1) and those haplotypes similar to IC1, M1 or P1 (Figure 2). To assess the genetic relatedness of pfcrt mutants, a haplotype network based on size variations at all MS markers was constructed. The haplotype network clearly showed three distinct clusters of pfcrt mutants (Figure 3). The first lineage (Indochina lineage) consisted of the most prevalent haplotype IC1 (n = 57), having a combination of alleles of 152-180-182-150-203-191 at the MS loci of -29.268 kb, -10.833 kb, -2.814 kb, 0.59 kb, 10.389 kb and 23.576 kb, respectively, and those haplotypes closely related to IC1. Nearly all isolates in this lineage harboured the CVIET genotype. However, several isolates (IC1, IC5, IC6, IC9 and IC10; n = 14) contained the CVIDT genotype. This indicates that this mutant genotype shares a common origin with CVIET, and that MS haplotype IC1 contained two mutant pfcrt genotypes. The second lineage (Melanesian lineage) contained the most prevalent haplotype M1 (n = 36), having an allele combination of 152-172-182-152-206-187 and those haplotypes related to M1. All but M2 (CVMNT, n = 3) harboured the S VMNT genotype. This indicates that MS haplotype M1 also contained two mutant pfcrt genotypes. In the third lineage (Philippine lineage), all but one (P2) harboured an allele combination of 152-170-190-142-200-189 (P1). As previously observed in the Melanesian lineage [1], all isolates in the Philippine lineage harboured the S VMNT genotype.

The geographical distribution of the three major lineages described above was clearly distinctive (Figure 4). The Indochina lineage was widely distributed in Indochina and Africa, and this is consistent with previous reports [1, 11]. Distribution of the Melanesian lineage was limited to Papua New Guinea and Vanuatu, except for four isolates (M1 and M2 found in the Philippines, which probably migrated from Melanesia).