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. 2021 Sep 27;28:67. doi: 10.1051/parasite/2021063

Artemisinin derivative-containing therapies and abnormal hemoglobin: Do we need to adapt the treatment?

Thérapies contenant des dérivés de l’artémisinine et hémoglobine anormale : faut-il adapter le traitement ?

Eric A Gbessi 1, Offianan A Toure 1, Albert Gnondjui 1, Tossea S Koui 1, Baba Coulibaly 1, Berenger A Ako 1, Nguessan L Tiacoh 1, Serge-Brice Assi 2, Ibrahima Sanogo 3, Didier-Paulin Sokouri 5, Ronan Jambou 1,4,*
PMCID: PMC8475499  PMID: 34569928

Abstract

Background: Artemisinin-based treatment in malaria patients with abnormal hemoglobin may be ineffective because of their genetic particularity, which could lead to resistance. The main purpose of this study was to assess the effect of artemisinin derivatives on in vivo parasite clearance according to erythrocyte variants. In vivo response was investigated through retrospective data obtained over a 42-day artemether-lumefantrine/artesunate amodiaquine efficacy protocol conducted from 2012 to 2016. Results: A total of 770 patients in Côte d’Ivoire attending the hospitals of Anonkoua-koute (Abidjan), Petit Paris (Korhogo), Libreville (Man), Dar es salam (Bouaké), Ayamé and Yamoussoukro with acute uncomplicated falciparum malaria were selected for successful hemoglobin typing. HbAS, HbSS, HbAC, and HbSC genotypes were found. Parasite clearance time was obtained for 414 patients. In the population with abnormal hemoglobin, parasite densities on admission and parasite clearance rates were significantly lower in the HbSC group compared to HbAA (p = 0.02 and p = 0.007, respectively). After PCR correction on day 42, the acute treatment rate was 100% for each group. Parasite half-life and time for initial parasitaemia to decline by 50 and 99% were longer for the HbSC group (p < 0.05). The study also investigated the prevalence of K13-propeller polymorphisms across different hemoglobin genotype groups. A total of 185 and 63 samples were sequenced in the HbAA group and patients with abnormal Hb, respectively. Only two nonsynonymous mutations D559N and V510M were found in the HbAA group. Conclusion: Although this study proved good efficacy of artemether-lumefantrine and artesunate amodiaquine in the treatment of uncomplicated Plasmodium falciparum malaria in patients with abnormal hemoglobin, the increased delay of parasite clearance may represent a threat to health in these patients in relation with sickle cell crisis, which could support selection of parasites resistant to artemisinin.

Keywords: Hemoglobinopathy, malaria, Ivory Coast, artemisinin containing therapy

Introduction

Hemoglobinopathies are inherited globin disorders [24] that affect 7% of the world population. 300,000 to 400,000 children are born each year with a severe form of the disease [28]. When glutamin is replaced by valin (6GAG > 6GTG), hemoglobin is called HbS (Hemoglobin S) and when replaced by lysine (6GAG > 6AAG), the abnormal hemoglobin is HbC (Hemoglobin C) [24]. In West Africa, the main mutation results in S or C variants of hemoglobin.

In addition to studies on thalassemia that have shown protection against malaria [11, 31] other studies focusing on HbS and HbC have shown that these abnormalities are involved in protection against malaria [2, 3, 13, 14]. This protection concerns not only malaria infection itself but mainly severe forms of malaria. Clinical responses of patients with hemoglobinopathy can differ according to host genetics [3, 7]. Although there is no difference in chloroquine metabolism, results published by Orjih in 1987 indicated that the hemoglobin genotype modulates the level of chloroquine in erythrocyte cells [16]. Another study showed that artesunate and chloroquine had less activity against Plasmodium falciparum growing in alpha-thalassemia and/or HbCS (Hb Constant Spring) erythrocytes than in normal erythrocytes, while the activity of pyrimethamine was the same for all erythrocytes. This could be due to an increased amount of antioxidant enzymes naturally found in abnormal erythrocytes, which could counterbalance the oxidative activity of artesunate [9, 32]. This suggests that patients with hemoglobinopathies may be at increased risk of inadequate response to artemisinin combination therapies (ACTs), especially in areas where parasite resistance or tolerance to artemisinin derivatives have emerged [18]. These results highlight the important role of hemoglobinopathy in parasite-host-drug interactions. However, very few studies address this question of the effects of erythrocyte variants on antimalarial efficacy. The 50% inhibitory concentration (IC50) of artesunate in normal and abnormal cells is used to assess its efficacy in vitro, and this concentration was found to be higher in abnormal cells [32]. In vivo, this efficacy can be measured by parasite clearance expressed as the parasite half-life in the patients’ blood. Using this parameter, the usual time to denote artemisinin resistance is 5 h [8].

A recent study in Ghana found that the parasite clearance in sickle cell disease (SCD) children with uncomplicated malaria was slower compared with clearance in non-SCD children, although artesunate-amodiaquine (AA) and artemether-lumefantrine (AL) showed similar clinical and parasitological effects in the SCD and non-SCD groups [1]. The World Health Organization has endorsed ACT as first‐line treatment where the potentially life‐threatening parasite Plasmodium falciparum is the predominant infecting species [6]. This strategy has been implemented in Côte d’Ivoire since 2005 [22], where the proportion of patients with abnormal hemoglobin attending dispensaries for malaria is largely unknown and probably underestimated. HbS and HbC genotypes were found in all the regions of Côte d’Ivoire with the highest prevalence (27%) in the Northern region [20].

The main purpose of this study was to assess in vivo the effect of artemisinin on parasite clearance according to erythrocyte variants. Data collected during in vivo drug efficacy surveys conducted on behalf of the National Malaria Control Program were analyzed retrospectively.

Materials and methods

Ethical considerations

Studies were conducted at all sites according to the declaration of Helsinki and national legal and regulatory requirements. Protocol, case report form, and informed consent form were approved by the “Comité National d’Éthique de la Recherche” of Côte d’Ivoire [21].

Study sites

During the past 8 years, six study sites were investigated in the country (Fig. 1). They are located in various ecological contexts, which can induce different levels of premunition and thus of parasitemia. Abidjan is the economic capital of the country accounting for almost 6 million inhabitants. It is located in the South of the country, with a sub-equatorial climate. Ayamé is located 100 km North–East of Abidjan, in a region of lakes. It is a tropical area where rainfalls almost all year and with a very high malaria transmission level. Yamoussoukro is the administrative capital, 248 km North of Abidjan, located in a region of lakes with an equatorial climate. Transmission of malaria is lower with rainfall of less than 900 mm/year. Man is the main town of the Western part of the country, 150 km from Yamoussoukro, surrounded by hills and dense forests. The climate is tropical and transmission of malaria is intense. Bouaké has 1 million inhabitants and is located 200 km North of Yamoussoukro, located in a savannah region. Korhogo is on the border with Mali and Burkina Faso. In these two latter places, the climate is typically sub-Sahelian (dry and hot) and malaria transmission is less intense than in other parts of the country [20].

Figure 1.

Figure 1

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Map of Côte d’Ivoire with site locations and prevalence of hemoglobin phenotypes.

Study population

The patients included in this study were recruited during therapeutic efficacy studies of ACTs, conducted on behalf of the National Malaria Control Program. Protocol of enrolment followed the 42 days WHO protocol [29].

Patients with microscopically confirmed acute uncomplicated falciparum malaria, parasite density ranging from 2000 to 200,000 asexual parasites/μL (both inclusive) and an axillary temperature ≥ 37.5 °C or history of fever in the past 24 h, were included in the study. Exclusion criteria included general signs of severe falciparum malaria according to the WHO definition. Patients with other plasmodium species than falciparum were not included, as well as patients already treated before attending the dispensary or patients unable to take oral medication.

Patients attending dispensaries for malaria suspicion were clinically examined and malaria was confirmed by Giemsa-stained thick smear examination. Patients received either AA or AL for 3 days under supervision by medical staff. Follow-up of patients through clinical investigation and blood sample was done during systematic outpatient visits at days 1, 2, 3, 7, 14, 21, 28, 35, and 42. Patients recruited in Ayamé and Bouaké were hospitalized for 3 days and followed-up at days 3, 7, 14, 21, 28, 35, and 42. During the first 3 days, thick blood smears were done every 6 h until two consecutive negative parasitemia results were obtained [22, 29]. Treatment failure was confirmed by microscopy examination of thick blood smears and defined either as “parasitological failure” if parasites are detected on the thick smear, or as “clinical failure” in case of presence of parasites on the thick smear plus fever. Early clinical failure, late clinical failure, and parasitological failure were defined as previously [29]. For all the patients with positive smear, blood samples were taken using EDTA-tubes and 50 μL were blotted on to Whatman 3 MM cards. Isolates from patients with treatment failure (but not those with treatment success) were genotyped using msp1 and msp2 nested-PCR to exclude new infection [29].

Hemoglobin typing

Two methods of hemoglobin typing were used according to the samples available. For samples from Yamoussoukro, Ayamé, and Korhogo, electrophoresis of hemoglobin was performed on Hydrasys® gel, following the manufacturer’s recommendations [23]. For blood samples collected on paper, typing was done using the FRET (fluorescence resonance energy transfer) approach after DNA extraction and PCR amplification [20].

K13-propeller genotyping and sequencing

DNA was extracted using a QiAamp® DNA kit, according to the manufacturer’s recommendations. DNA was stored at −20 °C. Plasmodium falciparum K13 gene was amplified and bi-directionally sequenced using the Sanger protocol by Genewiz institute. Sequences were aligned with the K13 P. falciparum 3D7 reference sequence (PF3D7-1343700) [4].

Statistical analysis

The number of patients enrolled by site was set as recommended by the WHO protocol [29]. At least 50 patients were registered for each arm (AA or AL). For 6 h and 24 h follow-up, parasite clearance was analyzed with the Antimalarial Resistance Network parasite clearance estimator (https://www.wwarn.org) and the WHO online parasite clearance estimator (http://www.who.int/malaria/areas/treatment/drug_efficacy/en/), respectively. For each group of patients with normal or abnormal hemoglobin, the time required for the decrease of X% of the initial parasitemia (PCx) was calculated. The parasite half-life was defined as the time required for the number of parasites in the peripheral blood (parasitemia) to decrease by 50%. It is derived from the slope of the linear part of the log-transformed parasitemia versus time curve. The clearance rate (k) was defined as the decrease of parasitemia per unit of time (per hour). Decreased response of treatment or the potential resistance of parasites are defined as the presence of parasites in blood on day 3 or by parasite half-life greater than 5 h. Pearson’s χ 2 test and Fisher’s exact test were used for comparison of proportions, whereas the Mann–Whitney test was used for parasite densities and parasite clearance data. Descendant logistic regression was used to define risk factors associated with the occurrence of treatment failures with p-value > 0.2 as cut-off of exclusion of the variables. Parameters used included region, parasitemia at day 0 (D0), gender, age, type of hemoglobin and parasitemia decay (quoted as more or less 5 h). Data analysis was done on R, version 3 environment and GraphPad Prism version 5. A p-value ≤ 0.05 was considered statistically significant.

Results

Population enrolled and parasitemia

Samples from 770 patients with uncomplicated malaria were analyzed for hemoglobin genotyping. Among them, 124 patients (16.1%) harbored abnormal hemoglobin (aHb). The aHb genotype distributions of these patients were: AC, n = 60 (7.79%); AS, n = 47 (6.10%); CC, n = 5 (0.64%); SC, n = 7 (0.90%) and, SS, n = 5 (0.64%). Patient mean age and the number of patients under 5 years old were similar in all groups (p > 0.05) (Table 1). Unlike patients with AC, AS and CC genotypes, parasite density at enrolment was lower in patients with SC genotype in comparison to the AA group (p = 0.02).

Table 1.

Baseline demographic characteristics.

HbAA HbAC HbAS HbCC HbSC HbSS
Characteristics at day 0 n (%) 646 60 47 5 7 5
 Age (years), mean (±SD) 12.7 (12.9) 13.5 (9.7) 14.9 (15.9) 11.0 (5.3) 12.7 (7.6) 10.8 (8.6)
 Age (<5 years), n (%) 177 (27.4) 13 (21.6) 14 (29.7) 0 (00) 0 (00) 2 (40.0)
 Sex, n (%) females 344 (53.2) 30 (50) 27 (57.4) 4 (80.0) 4 (57.1) 2 (40.0)
 Pf parasitemia (/μL of blood), median (IQR) 28,978 (7982–72,000) 20,052 (5980–68,156) 17,280 (4644–82,400) 27,394 (25,000–34,690) 8400 (3654–16,650) 15,700 (14,892–24,000)
p-values HbAA vs. HbAC HbAA vs. HbAS HbAA vs. HbCC HbAA vs. HbSC HbAA vs. HbSS
 Age (years), mean (±SD) 0.07 0.58 0.55 0.41 0.93
 Age (<5 years), n (%) 0.36 0.73 0.33 0.19 0.61
 Sex, n (%) females 0.68 0.65 0.37 1 0.69
 Pf parasitemia (/μL of blood), median (IQR) 0.15 0.40 0.97 0.02 0.56
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Abbreviations: Hb, hemoglobin; Pf., Plasmodium falciparum; SD, standard deviation; μL, microliter; IQR, interquartile range.

Parasite clearance

Parasite clearance was estimated for 414 patients. In this study, the median parasite clearance time (PCT) varied between 24 and 48 h, with 24 h for AA, AC, AS and SS genotypes against 48 h for CC and SC genotypes. In general, there was no difference between the PCT of normal hemoglobin (nHb) compared to abnormal hemoglobin (aHb) (nHb: 32.6 h ± 12.5; aHb: 32.3 h ± 12.8, p = 0.68). Specifically, the PCT was thus longer for patients with CC and SC genotypes than for AA genotype, where differences were only significant between SC and AA groups (p = 0.02). Patients with HbSC, had a longer parasite half-life time (clearance 50%) (p = 0.008) and a lower parasite clearance rate (p = 0.007) than those with AA hemoglobin (Table 2). Proportion of isolates potentially resistant, proportion of patients with parasitemia at days 3 > 10% of the day 0 (Table 3), and the number of patients with a slope half-life > 5 h (Table 2), were not different for patients with or without aHb (p = 1). Acute clinical and parasitological response (ACPR) rates on day 42 were similar in all groups (100%) (Table 3).

Table 2.

Characteristics of parasite clearance according to hemoglobin type.

HbAA HbAC HbAS HbCC HbSC HbSS
Patients for parasite clearance calculation (n)* 359 20 22 4 6 3
 Median k (/hour), (IQR) 0.2 (0.2–0.3) 0.2 (0.2–0.2) 0.2 (0.2–0.3) 0.2 (0.1–0.2) 0.1 (0.1–0.2) 0.2 (0.1–0.2)
 Slope half-life (hour), median (IQR) 3.1 (2.7–3.6) 2.9 (2.7–3.2) 2.6 (2.3–3.6) 3.4 (3.2–3.6) 3.8 (3.6–3.9) 3.2 (2.5–4.3)
 Patients with slope half-life > 5 h, n (%) 26 (7.2) 1 (5.0) 1 (4.5) 0 0 0
 PCT in hours, median (IQR) 24 (24–48) 24 (24–36) 24 (24–48) 48 (42–48) 48 (48–48) 24 (24–48)
 PC50, median (IQR) 12.1 (9.4–13.3) 11.9 (8.2–12.4) 11.7 (9.2–13.9) 12.8 (12.5–13.1) 13.7 (13.6–14.0) 12.5 (9.2–14.4)
 PC90, median (IQR) 21.9 (14.7–23.7) 21.7 (14.5–22.6) 20.3 (13.3–23.9) 23.4 (22.9–23.9) 24.8 (24.2–25.1) 22.9 (15.0–26.2)
 PC95, median (IQR) 24.9 (17.3–27.0) 24.8 (17.3–25.7) 23.2 (15.1–27.3) 26.7 (26.1–27.3) 28.3 (27.6–28.6) 26.1 (17.5–29.9)
 PC99, median (IQR) 31.0 (23.0–33.6) 30.7 (23.7–31.9) 28.8 (19.2–33.9) 33.1 (32.3–33.8) 35.0 (34.2–35.4) 32.3 (23.4–36.9)
p-values HbAA vs. HbAC HbAA vs. HbAS HbAA vs. HbCC HbAA vs. HbSC HbAA vs. HbSS
 Median k (/hour), (IQR) 0.44 0.80 0.16 0.007 0.54
 Slope half-life (hour), median (IQR) 0.89 0.87 0.18 0.008 0.56
 PCT in hours, median (IQR) 0.13 0.49 0.05 0.02 0.82
 PC50, median (IQR) 0.34 0.74 0.24 0.006 0.65
 PC90, median (IQR) 0.56 0.83 0.13 0.01 0.53
 PC95, median (IQR) 0.55 0.82 0.12 0.02 0.14
 PC99, median (IQR) 0.64 0.86 0.15 0.03 0.54
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Notes: PC50, 50% parasite clearance rate; PC90, 90% parasite clearance rate; PC95, 95% parasite clearance rate; PC99, 99% parasite clearance rate.

*

Parasite clearance was estimated by WWARN PCE and WHO PCE.

Abbreviations: Hb, hemoglobin; IQR, interquartile range; PCE, parasite clearance estimator; PCT, parasite clearance time; k, parasite clearance rate.

Table 3.

Characteristics of patients during follow-up according to hemoglobin type.

HbAA HbAC HbAS HbCC HbSC HbSS
Patients followed-up from day 3 onward (n) 646 60 47 5 7 5
 Positive parasitemia on day 3 n (%) 3 (0.5) 1 (1.7) 0 (00) 0 (00) 0 (00) 0 (00)
 Early treatment failure (ETF) n (%) 0 (00) 0 (00) 0 (00) 0 (00) 0 (00) 0 (00)
 Late clinical failure (LCF) n (%) 33 (5.1) 4 (6.7) 1 (2.1) 1 (20) 0 (00) 0 (00)
 Late parasitological failure (LPF) n (%) 7 (1.1) 0 (00) 0 (00) 0 (00) 0 (00) 0 (00)
 Recrudescence (defined on PCR typing) n (%) 0 (00) 0 (00) 0 (00) 0 (00) 0 (00) 0 (00)
 New infection n (%) 40 (6.2) 4 (6.7) 1 (2.1) 1 (20) 0 (00) 0 (00)
 Adequate clinic parasitological response (ACPR) (%) 100 100 100 100 100 100
p-values HbAA vs. HbAC HbAA vs. HbAS HbAA vs. HbCC HbAA vs. HbSC HbAA vs. HbSS
 Positive parasitemia on day 3 n (%) 0.29 1 1 1 1
 Early treatment failure (ETF) n (%) 1 1 1 1 1
 Late clinical failure (LCF) n (%) 0.54 0.72 0.23 1 1
 Late parasitological failure (LPF) n (%) 1 1 1 1 1
 Recrudescence (defined on PCR typing) n (%) 1 1 1 1 1
 New infection n (%) 0.78 0.35 0.27 1 1
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However, when time for parasite half-life time of each patient is plotted as histogram and analyzed according to White et al. [27], different distributions of parasite population can be highlighted (Fig. 2): i) for patients with aHb, only one parasite population with a mean half-life time at 2.15 ± 1.37 h (sensitive to ACT), ii) for patients with nHb three populations of parasites can be predicted with half-life time at 1.83 ± 1.28 h for 25.4% of the patients, 3.23 ± 1.17 h for 66.9% of the patients, and 7.78 ± 1.32 h for 7.7% of the patients (Fig. 1). This last group can be considered “ACT low sensitivity”.

Figure 2.

Figure 2

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Modeling the population parasite number according to the hemoglobin type. The parasite half-life time is plotted for those with (A) or without (B) abnormal hemoglobin according to the White et al. [27], distribution model. For aHb, the model describes only one phenotype (half-life time = 2.15 ± 1.37 h), whereas for nHb, three phenotypes were found: i) phenotype 1 (blue line, half-life time = 1.83 ± 1.28 h) accounting for 25.4% of the patients, ii) phenotype 2 (red line, half-life time = 3.23 ± 1.17 h) accounting for 66.88% of the patients, and iii) phenotype 3 (pink line, half-life time = 7.78 ± 1.32 h) accounting for 7.73%. The red line highlights the threshold of potential resistance (half-life more than > 5 h). aHb (Abnormal hemoglobin), nHb (Normal hemoglobin).

Parameters linked to drug failure

A logistic regression model was used to search for parameters linked with the risk of treatment failure (both parasitological LPF and clinical failure ETF/LCF). The model stopped with Wald test at 31.84 (4 df, p = 2.066e−06). Only the age group (age < 5 years, odds ratio [OR = 5.74], p < 0.0001), the half-life of parasite decay more than 5 h (OR = 3.69, p = 0.01) and HbCC genotype (OR = 11.74, p = 0.04) were significantly linked with the risk of failure (Table 4).

Table 4.

Multivariate analysis of risk factors associated with the occurrence of treatment failures.

Logistic model Failure (%) Odds ratio [CI 95%] p-value
Half-life (hours)
 < 5 h 40 (10.4) 1
 > 5 h 6 (21.4) 3.69 [1.18–10.3] 0.01
Hemoglobin type
 AA 40 (6.2) 1
 AC 4 (6.7) 1.5 [0.21–6.25] 0.62
 AS 1 (2.1) 0.54 [0.02–2.94] 0.56
 CC 1 (20.0) 11.74 [0.54–104] 0.04
 SC 0 (0.0) 0 0.99
 SS 0 (0.0) 0 0.99
Gender
 Female 18 (4.4) 1
 Male 28 (7.8) 1.57 [0.72–3.53] 0.25
Age group
 ≥ 5 years 16 (2.8) 1
 < 5 years 30 (14.6) 5.74 [2.6–13.1] 0.0001
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Notes: Logistic regression stopped with Wald test 31.84 on 4 df (p = 2.066e−06). Only the variables age group (age < 5 years), parasite half-life, and HbCC were significantly linked with the risk of failure.

K13-propeller genotypes

Overall, 247 sequences were obtained for the K13-propeller gene, 63 sequences for aHb and185 sequences for nHb. These sequences derived from parasite isolates with density greater than 10,000/μL of blood. Height mutations were detected out of which only two were non-synonymous (D559N and V510M). These non-synonymous mutations were found in isolates from people with nHb. Only one synonymous mutation was found in isolates from patients with aHb (1.61%) (Table 5).

Table 5.

Prevalence of K13-propeller gene mutations according to hemoglobin type.

HbAA HbAC HbAS HbCC HbSC HbSS
Sequences obtained (n) 185 27 22 05 04 05
 Sequences WT, n (%) 178 (96.2) 24 (100) 22 (100) 05 (100) 04 (100) 04 (80.0)
 Mutated sequences, n (%) 07 (3.8) 0 (00) 0 (00) 0 (00) 0 (00) 01 (20)
Nature of mutation
 Synonymous mutations, n (%) 05 (2.70) 01 (20)
 Non-synonymous mutations, n (%) 02 (1.08)
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Notes: Synonymous mutations (HbAA: Y519Y R597R V510V T535T C469C, HbSS: C469C); Non-synonymous mutations (HbAA: D559N V510M).

Abbreviations: WT, wild type; Hb, hemoglobin.

Discussion

This study focuses on parasite clearance in patients with hemoglobin disorders. The in vivo effect of ACTs on parasites was evaluated in patients who attended consultation without prior knowledge of their hemoglobin status. From 2012 to 2016, two protocols of follow-up were used on behalf of the National Malaria Program to survey drug efficacy, for a 24-hour follow-up and a 6-hour follow-up.

For the 770 patients enrolled in this study in 6 provinces, a significantly lower initial parasite density was found in HbSC genotype patients, compared with HbAA group, as previously reported [7, 19, 26]. According to the literature, this was related to a lack of maturation of parasites in sickle cells, an increase in phagocytosis of infected red blood cells, or more recently, to the effect of human microRNA on the intracellular control of the parasite [14, 20]. In this study, during treatment, a lower clearance rate, a longer time to 50% and 99% parasite clearance, and a longer parasite half-life were found for people with HbSC than for HbAA patients, but not for other types of hemoglobin. Previous in vitro results have shown that artesunate and chloroquine had less activity against P. falciparum growing in alpha-thalassemia and/or HbCS erythrocytes than normal erythrocytes, while the activity of pyrimethamine was the same for all erythrocytes [32]. Clearly, these data support evidence that hemoglobinopathies modulate the activity of artemisinin derivatives. Authors attribute these results to altered accumulation and lower binding of molecules within the parasitized erythrocytes as well as attenuation of oxidative stress [17, 18]. Antagonistic actions of erythrocyte antioxidative enzymes [17] and artesunate oxidative activity [5] could lead to this higher clearance time in abnormal erythrocytes. However, the low initial parasite density found in these patients with HbSC genotype could have led us to expect even faster parasite clearance. These results show that normal and abnormal blood cells have significantly different biochemistry.

However, the best measure of parasite clearance is the parasite half-life in a patient’s blood. The usual threshold used for artemisinin resistance is 5 h. This definition complements the WHO definition arguing that artemisinin resistance must be suspected in a population if more than 10% of patients continue to carry parasites 3 days after beginning of ACT treatment [27]. Globally, this study showed no failure difference between patients with or without aHb. The same applies for the various therapeutic failure criteria (ET, LC, LPF). Indeed, in logistic regression, the main factors associated with failure were, parasite half-life time “> 5 h”, group of “age < 5 years”, and homozygote “HbCC genotype”.

This last parameter is interesting as HbC is mainly a Sahelian genetic trait and two studies demonstrated the malaria protective effect of this hemoglobin. Agarwal et al. studying a Dogon population with a high prevalence of HbC, reported that subjects with HbAC were 29% less likely to develop severe malaria than subjects with HbAA [2]. One year later, in Burkina Faso, a study confirmed that HbC was associated with about 90% reduced risks of malaria (both mild and severe) [14]. Recently, a study implemented in Mali, indicated that schoolchildren with hemoglobin C mutation might contribute disproportionately to the seasonal malaria resurgence in an area where the HbC variant is common, related to an increase of asymptomatic carriage of parasites [10]. Data obtained during this study in Côte d’Ivoire support this last point and add rational to additional effects of HbC on malaria epidemiology, with delayed efficacy of artemisin derivatives (ART) for these patients.

Artemisinin resistance monitoring remains a priority for the National Malaria Control Program of Cote d’Ivoire because of the threat of import of resistant strains from Asian countries [15, 30]. Genetic analysis of populations of parasites is thus an important tool to conduct retrospective surveys. The A578S mutation observed in Yunnan province, China associated with the predominant F446I mutation [19], has already been reported in some African countries [12]. In this study, two new nonsynonymous mutations (D559N and V510M) were found in patients with nHb, not related to Southeast Asia ones [19], without association with abnormal hemoglobin or delay response. However, at the same time, an analysis conducted by White et al. [25, 27] supports different structures of parasite populations for patients with aHb and nHb. This could suggest higher biochemical constraints for the development of the parasite in aHb. Interestingly, in abnormal cells, constraints in parasite growth significantly reduce biomass and therefore can affect the phenotypic diversity of parasites. The second hypothesis could be that aHb can selects specific phenotypes usually at low frequency in the parasite population. Given the high frequency of people living with aHb in Côte d’Ivoire, this could place considerable pressure on parasites, supporting emergence of drug resistance (as resistance to ART seems related to anti-oxidant metabolism).

In conclusion, despite the significant delay in parasitic clearance observed in HbSC patients compared to HbAA patients, the ACTs remain highly effective in these patients. This is good news for the National Malaria Control Program, as patients with any type of hemoglobin will be able to use the same antimalarial drug. However, the high homogeneity of the isolates invading aHb patients suggests a specific genetic background in these parasites. Full genome sequencing of these isolates is now in progress.

Acknowledgments

We are grateful to the participants, medical staff, and all health authorities at the study sites for their collaboration. The authors would also like to acknowledge the National Malaria Control Program (PNLP-CI), WHO, Global Fund and Rotary International.

Cite this article as: Gbessi EA, Toure OA, Gnondjui A, Koui TS, Coulibaly B, Ako BA, Tiacoh NL, Assi S, Sanogo I, Sokouri D & Jambou R. 2021. Artemisinin derivative-containing therapies and abnormal hemoglobin: Do we need to adapt the treatment? Parasite 28, 67.

Conflict of interest

The authors declare that they have no competing interests.

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