ABSTRACT
Malaria is an acute febrile disease caused by a protozoan of the genus Plasmodium. Light microscopy (LM) is the gold standard for the diagnosis of malaria. Despite this method being rapid and inexpensive, it has a low limit of detection, which hampers the identification of low parasitemia infections. By using multicopy targets and highly sensitive molecular techniques, it is possible to change this scenario. In this study, we evaluated the performance of droplet digital PCR (ddPCR) to detect Plasmodium DNA obtained from saliva samples (whole saliva and buccal swab) of 157 individuals exposed to malaria transmission from the Brazilian Amazon region. We used the highly sensitive ddPCR method with non-ribosomal multicopy targets for Plasmodium vivax (Pvr47) and Plasmodium falciparum (Pfr364). There was good concordance between the quantitative real-time PCR (qPCR) results from the saliva and blood, except for mixed-species infections. The sensitivity of qPCR was 93% for blood, 77% for saliva, and 47% for swabs. Parasite DNA was not detected in saliva samples in low-density infections compared with the detection in blood samples. ddPCR showed increased sensitivity for detecting Plasmodium in the blood and swabs (99% in blood, 73% in saliva, and 59% in swabs). Notably, ddPCR detected more mixed infections in the blood (15%), saliva (9%), and swabs (18%) than qPCR. Our data showed that the differences between ddPCR and qPCR were the result of a higher number of P. falciparum infections detected by ddPCR. Overall, there was a moderate correlation between parasite densities estimated by the different methods in the blood. Our findings highlight the possibility of using non-invasive sample collection methods for malaria diagnosis by targeting multicopy sequences combined with highly sensitive molecular methods.
ABSTRACT
Early diagnosis and treatment are fundamental to the control and elimination of malaria. In many endemic areas, routine diagnosis is primarily performed microscopically, although rapid diagnostic tests (RDTs) provide a useful point-of-care tool. Most of the commercially available RDTs detect histidine-rich protein 2 (HRP2) of Plasmodium falciparum in the blood of infected individuals. Nonetheless, parasite isolates lacking the pfhrp2 gene are relatively frequent in some endemic regions, thereby hampering the diagnosis of malaria using HRP2-based RDTs. To track the efficacy of RDTs in areas of the Brazilian Amazon, we assessed pfhrp2 deletions in 132 P. falciparum samples collected from four malaria-endemic states in Brazil. Our findings show low to moderate levels of pfhrp2 deletion in different regions of the Brazilian Amazon. Overall, during the period covered by this study (2002-2020), we found that 10% of the P. falciparum isolates were characterized by a pfhrp2 deletion. Notably, however, the presence of pfhrp2-negative isolates has not been translated into a reduction in RDT efficacy, which in part may be explained by the presence of polyclonal infections. A further important finding was the discrepancy in the proportion of pfhrp2 deletions detected using two assessed protocols (conventional PCR versus nested PCR), which reinforces the need to perform a carefully planned laboratory workflow to assess gene deletion. This is the first study to perform a comprehensive analysis of PfHRP2 sequence diversity in Brazilian isolates of P. falciparum. We identified 10 PfHRP2 sequence patterns, which were found to be exclusive of each of the assessed regions. Despite the small number of PfHRP2 sequences available from South America, we found that the PfHRP2 sequences identified in Brazil and neighboring French Guiana show similar sequence patterns. Our findings highlight the importance of continuously monitoring the occurrence and spread of parasites with pfrhp2 deletions, while also taking into account the limitations of PCR-based testing methods associated with accuracy and the complexity of infections.
Subject(s)
Malaria, Falciparum , Plasmodium falciparum , Antigens, Protozoan/genetics , Brazil , Diagnostic Tests, Routine , Gene Deletion , Histidine , Humans , Malaria, Falciparum/diagnosis , Plasmodium falciparum/genetics , Protozoan Proteins/geneticsABSTRACT
BACKGROUND: The resistance of Plasmodium vivax to chloroquine has become an obstacle to control strategies based on the use of anti-malarials. The current study investigated the association between P. vivax CQ-resistance in vivo with copy number variation and mutations in the promoter region in pvcrt-o and pvmdr1 genes. METHODS: The study included patients with P. vivax that received supervised treatment with chloroquine and primaquine. Recurrences were actively recorded during this period. RESULTS: Among the 60 patients with P. vivax, 25 were CQ-resistant and 35 CQ-susceptible. A frequency of 7.1% of multi-copy pvcrt-o was observed in CQ-susceptible samples and 7.7% in CQ-resistant at D0 (P > 0.05) and 33.3% in CQ-resistant at DR (P < 0.05). For pvmdr1, 10.7% of the CQ-susceptible samples presented multiple copies compared to 11.1% in CQ-resistant at D0 and 0.0% in CQ-resistant at DR (P > 0.05). A deletion of 19 bp was found in 11/23 (47.6%) of the patients with CQ-susceptible P. vivax and 3/10 (23.1%) of the samples with in CQRPv at D0. At day DR, 55.5% of the samples with CQRPv had the 19 bp deletion. For the pvmdr-1 gene, was no variation in the analysed gene compared to the P. vivax reference Sal-1. CONCLUSIONS: This was the first study with 42-day clinical follow-up to evaluate the variation of the number of copies and polymorphisms in the promoter region of the pvcrt-o and pvmdr1 genes in relation to treatment outcomes. Significantly higher frequency of multi-copy pvcrt-o was found in CQRPv samples at DR compared to CQ-susceptible, indicating parasite selection of this genotype after CQ treatment and its association with CQ-resistance in vivo.
Subject(s)
Antimalarials/pharmacology , Chloroquine/pharmacology , DNA Copy Number Variations/drug effects , Drug Resistance , Membrane Transport Proteins/genetics , Plasmodium vivax/drug effects , Protozoan Proteins/genetics , Adolescent , Adult , Brazil , Child , Child, Preschool , Female , Humans , Infant , Malaria, Vivax/prevention & control , Male , Membrane Transport Proteins/metabolism , Middle Aged , Mutation , Plasmodium vivax/genetics , Polymorphism, Genetic , Protozoan Proteins/metabolism , Young AdultABSTRACT
[This corrects the article DOI: 10.1371/journal.pone.0160172.].
ABSTRACT
BACKGROUND: Parasite resistance to anti-malarials represents a great obstacle for malaria elimination. The majority of studies have investigated the association between single-nucleotide polymorphisms (SNPs) and drug resistance; however, it is becoming clear that the copy number variation (CNV) is also associated with this parasite phenotype. To provide a baseline for molecular surveillance of anti-malarial drug resistance in the Brazilian Amazon, the present study characterized the genetic profile of both markers in the most common genes associated with drug resistance in Plasmodium falciparum and Plasmodium vivax isolates. Additionally, these data were compared to data published elsewhere applying a systematic review of the literature published over a 20-year time period. METHODS: The genomic DNA of 67 patients infected by P. falciparum and P. vivax from three Brazilian States was obtained between 2002 and 2012. CNV in P. falciparum multidrug resistance gene-1 (pfmdr1), GTP cyclohydrolase 1 (pfgch1) and P. vivax multidrug resistance gene-1 (pvmdr1) were assessed by real-time PCR assays. SNPs in the pfmdr1 and pfcrt genes were assessed by PCR-RFLP. A literature search for studies that analysed CNP in the same genes of P. falciparum and P. vivax was conducted between May 2014 and March 2017 across four databases. RESULTS: All analysed samples of P. falciparum carried only one copy of pfmdr1 or pfgch1. Although the pfcrt K76T polymorphism, a determinant of CQ resistance, was present in all samples genotyped, the pfmdr1 N86Y was absent. For P. vivax isolates, an amplification rate of 20% was found for the pvmdr1 gene. The results of the study are in agreement with the low amplification rates for pfmdr1 gene evidenced in the Americas and Africa, while higher rates have been described in Southeast Asia. For P. vivax, very low rates of amplification for pvmdr1 have been described worldwide, with exceptions in French Guiana, Cambodia, Thailand and Brazil. CONCLUSIONS: The present study was the first to evaluate gch1 CNV in P. falciparum isolates from Brazil, showing an absence of amplification of this gene more than 20 years after the withdrawal of the Brazilian antifolates therapeutic scheme. Furthermore, the rate of pvmdr1 amplification was significantly higher than that previously reported for isolates circulating in Northern Brazil.
Subject(s)
Drug Resistance , Gene Dosage , Plasmodium falciparum/genetics , Plasmodium falciparum/isolation & purification , Plasmodium vivax/genetics , Plasmodium vivax/isolation & purification , Protozoan Proteins/genetics , Adult , Brazil , Female , Gene Frequency , Humans , Male , Middle Aged , Polymorphism, Restriction Fragment Length , Polymorphism, Single Nucleotide , Real-Time Polymerase Chain ReactionABSTRACT
Um dos maiores desafios do controle da malária é a resistência do parasito aos antimaláricos. A biologia molecular tem permitido a compreensão desse fenótipo com o estudo de marcadores associados a ela, tais como o Polimorfismo de Base Única (SNP) e o Polimorfismo de Variação de Número de Cópias Gênicas (CNV). Alterações gênicas atribuídas ao CNV podem levar a alterações fenotípicas no parasito, conferindo resistência ou suscetibilidade aos antimaláricos. Sua presença foi relacionada com a falha terapêutica a drogas como cloroquina (CQ) e mefloquina (MQ) em diversas regiões do mundo. Os genes pfmdr1 e pfgch1 de P. falciparum e pvmdr1 de P. vivax são relacionados com resistência a diferentes fármacos. Entretanto, no Brasil poucos estudos caracterizaram esses genes quanto à presença de CNVs, sendo que sua maioria investigou a diversidade genética associada aos SNPs. O objetivo deste estudo foi investigar a presença de CNV nos genes pfmdr1 e pfgch1 de P. falciparum e pvmdr1 e pvcrt-o de P. vivax, assim como SNPs nos genes pfcrt e pfmdr1 de P. falciparum. O CNV foi determinado por qPCR utilizando sondas de hidrólise e os SNPs por PCR-RFLP. As amostras foram coletadas entre 2002 a 2012, em 3 diferentes estados brasileiros Mato Grosso (n=31), Rondônia (n=27) e Amapá (n=10)
As 31 amostras analisadas de P.falciparum apresentaram cópia única para pfmdr1 e pfgch1, apesar do histórico de resistência do parasito a vários antimaláricos utilizados ao longo do tempo no Brasil. Entretanto, um importante SNP em pfcrt (K76T), relacionado com resistência à CQ, foi identificado em todas as amostras analisadas. Nesse estudo, também foram analisados 38 isolados de P. vivax, sendo reportado a amplificação gênica em 7 (18%) amostras para pvmdr1. No sudoeste asiático altas taxas de CNV em pvmdr1 foram reportadas (38%), sendo relatado por um único estudo no Brasil (0,9% de amplificação). Um resultado importante desse estudo foi a observação, pela primeira vez, da amplificação de pvcrt-o. Embora estudos anteriores o associem com resistência e casos graves da doença, nenhum avaliou a presença de CNV em pvcrt-o. Este estudo é um dos primeiros a avaliar a presença de CNV nos genes pvmdr1, pvcrt-o e pfgch1 no Brasil, assim como estudar a distribuição de CNV no mundo através de uma revisão sistemática
Subject(s)
Male , Female , Humans , Drug Resistance , Malaria/drug therapy , PlasmodiumABSTRACT
Although Plasmodium vivax relapses are classically associated with hypnozoite activation, it has been proposed that a proportion of these cases are due to primaquine (PQ) treatment failure caused by polymorphisms in cytochrome P-450 2D6 (CYP2D6). Here, we present evidence that CYP2D6 polymorphisms are implicated in PQ failure, which was reinforced by findings in genetically similar parasites, and may explain a number of vivax relapses. Using a computational approach, these polymorphisms were predicted to affect the activity of CYP2D6 through changes in the structural stability that could lead to disruption of the PQ-enzyme interactions. Furthermore, because PQ is co-administered with chloroquine (CQ), we investigated whether CQ-impaired metabolism by cytochrome P-450 2C8 (CYP2C8) could also contribute to vivax recurrences. Our results show that CYP2C8-mutated patients frequently relapsed early (<42 days) and had a higher proportion of genetically similar parasites, suggesting the possibility of recrudescence due to CQ therapeutic failure. These results highlight the importance of pharmacogenetic studies as a tool to monitor the efficacy of antimalarial therapy.
