Background
Emergence and spread of
Plasmodium falciparum resistance to chloroquine (CQ) and sulfadoxine-pyrimethamine (SP) forced the adoption of artemisinin-based combination therapy (ACT) as first-line anti-malarial drugs in most sub-Saharan African countries (SSA) by 2007 [
1]. Since the introduction of ACT, SP has remained the combinational drug for ACT (SP-artesunate) used in a few SSA countries, or as a prophylactic drug in intermittent preventive treatment of malaria during pregnancy (IPTp) where three or more treatment doses of SP are administered on a monthly basis after the first trimester. SP as a prophylaxis is also used in infancy (IPTi) and as a seasonal malaria chemoprevention (SMC) in children [
2‐
4]. SMC in particular, where SP is combined with amodiaquine, is currently being implemented in West African countries (Chad, The Gambia, Niger, Mali, Senegal, Guinea) [
5], and it has been shown to be cost effective in reducing childhood morbidity and mortality due to malaria [
6].
SP acts by inhibiting the folic acid synthesis in the malaria parasite; sulfadoxine and pyrimethamine inhibit the
Plasmodium falciparum enzymes dihydropteroate synthetase (DHPS) and dihydrofolate reductase (DHFR), respectively [
7,
8]. Resistance to sulfadoxine and pyrimethamine is caused by mutations in the
P. falciparum
dhps and
dhfr genes, respectively.
Pfdhfr single-point mutations causing amino acid changes in N51I, C59R and S108 N are the most common mutations associated with pyrimethamine resistance in SSA [
9,
10] and the combination of these forming the triple
Pfdhfr IRN mutation is highly prevalent in SSA [
11,
12]. Regarding sulfadoxine resistance,
Pfdhps mutations S436A/C/F, A437G, K540E, A581G, and A613S/T have been observed globally [
13,
14] and S436A/C/F, A437G and G540E are commonly observed in SSA [
11]. The combination of the
Pfdhfr triple and the
Pfdhps double (A437G, K540E) mutations collectively form the quintuple mutations [
7,
15] which confers high-level SP resistance and is a significant predictor of SP
P. falciparum treatment failure [
16‐
18]. The evolution of the
Pfdhps mutations normally occurs after the
Pfdhfr triple mutations and thus the presence of
Pfdhps double mutations indicates presence of quintuple mutations.
In SSA, the highest prevalence of SP resistance markers has been documented in East Africa where the quintuple mutation has been shown to approach fixation [
12]. Evidence shows that the quintuple mutation emerged in the 1990s and in Tanzania as high as over 60 % was detected in 1998 [
19], while a recent survey documented more than 95 % quintuple mutation, in 2011 [
20]. In 2010, the World Health Organization (WHO), through its malaria advisory committee made a recommendation that SP-IPTi should be implemented only in areas where prevalence of the quintuple mutation, as represented by the
Pfdhps 540E, is less than 50 % [
21]. Given the high prevalence of the 540E in East Africa, this policy has led to the restricted recommendation of SP-IPTi to West Africa where the 540E mutation (and hence the quintuple mutation) is low or absent [
11]; currently, SP-IPTi is only implemented in Chad [
5].
In areas where the quintuple mutation is high, IPTp with SP does not prevent placental malaria but may continue to protect against severe pregnancy outcomes [
22‐
25]. WHO has continued to recommend use of at least three SP-IPTp doses even in such areas where the quintuple mutations are high [
26].
The emergence of an additional
Pfdhps mutation that is 581G in areas where the quintuple mutant is well established has been documented in two major foci in East Africa [
12]. Furthermore, in Tanzania in particular, the prevalence of the 581G has reached 55 % in the northeast [
27]. Growing evidence from studies performed mainly in Tanzania indicates that presence of the
Pfdhps 581G (sextuple mutant parasites), is associated with reduced SP-IPTp efficacy by: (1) a reduction in the protection period of SP-IPTp from 4 to 2 weeks [
23]; (2) increased parasitaemia [
23,
28] and recently, from a study in Malawi [
29], also increased placental parasitaemia [
28]; (3) increased risk of severe malaria in offspring [
30]; and, (4) low birth weight in new-borns from mothers undergoing SP-IPTp in Tanzania [
31]. Thus, the emergence of sextuple mutants seems to have a direct impact on the efficacy of the IPTp using SP. The existing information on the 581G distribution in Tanzania is scarce, mainly confined to the region of Tanga, and may not be evenly distributed across the country. A recent systematic review and meta-analysis of the influence of the
Pfdhps 581G mutation on SP-IPTp has shown that when the prevalence of 581G is >10 %, IPTp with SP does not protect against low birth weight [
32]. For a proper, evidence-based implementation of IPTp programme and an understanding of regions where the strategy may be compromised, a countrywide monitoring of the mutations is important. This study reports on the status of
Pfdhps K540E and A581G in Tanzania.
Methods
Filter paper blood spot, whole blood and used malaria rapid diagnostic test strips collected in previous studies between June 2010 and August 2011 in seven regions of mainland Tanzania were used for this study, as previously described [
33]. The study sites included Mwanza (Misungwi district) and Kagera (Muleba district) around Lake Victoria in the northwestern zone, Tanga (Muheza and Bondo) in the northeastern zone, Mtwara (Tandahimba and Mtwara-Urban), Coastal Region (Kibiti-Rufiji) and Lindi Region (Nachingwea) in the southeastern zone and Mbeya (Kyela and Rungwe districts) in the southwestern zone. The DNA samples were extracted using Chelex-100 method [
34]. Genotyping for
Pfdhps K540E and A581G was performed using polymerase chain reaction-restriction fragment length polymorphisms (PCR-RFLP) and polymerase chain reaction-single strand oligonucleotide probes-enzyme linked immunosorbent assay (PCR-SSOP-ELISA) methods described by others [
35‐
37]. All PCR reagents and restriction endonucleases were purchased from New England Biolabs (Ipswich, MA, USA). Primers were purchased from Biolegio (Nijmegen, The Netherlands). Prevalence was calculated for each genotype, excluding mixed infections in both individual genotype prevalence and in 540-581 haplotype analysis. Only a few mixed infections were observed in A581G (Table
1). Maps were constructed using ArcGIS version 10.2. The study received ethical approval from the Kilimanjaro Christian Medical University College Research Ethics Review Committee.
Table 1
Distribution of Pfdhps K540E and A581G polymorphisms among regions in Tanzania
Mwanza | Misungwi | 4 (3.0) | 129 (97.0) | 0 | 133 | 118 (95.2) | 6 (4.8) | 0 | 124 | 4 (3.2) | 0 (0.0) | 114 (91.9) | 6 (4.8) | 124 |
Mbeya | Multiple sites | 3 (2.0) | 150 (98.0) | 0 | 153 | 143 (93.5) | 9 (5.9) | 1 (0.7) | 153 | 3 (2.0) | 0 (0.0) | 140 (92.1) | 9 (5.9) | 152 |
Mtwara | Tandahimba and Mtwara urban | 30 (36.1) | 53 (63.9) | 0 | 83 | 76 (95.2) | 4 (4.8) | 0 | 80 | 29 (34.9) | 1 (1.2) | 50 (60.2) | 3 (3.6) | 83 |
Lindi | Nachingwea | 24 (27.3) | 64 (72.7) | 0 | 88 | 88 (100) | 0 | 0 | 88 | 24 (27.3) | 0 (0.0) | 64 (72.7) | 0 (0.0) | 88 |
Tanga | Bondo | 10 (8.6) | 106 (91.4) | 0 | 116 | 46 (40.6) | 64 (56.6) | 3 (2.7) | 113 | 7 (6.4) | 4 (3.6) | 39 (35.5) | 60 (54.5) | 110 |
Muheza | 5 (5.7) | 83 (94.3) | 0 | 88 | 43 (48.9) | 45 (51.1) | 0 | 88 | 5 (5.7) | 0 (0.0) | 38 (43.2) | 45 (51.1) | 88 |
Pwani | Rufiji | 23 (23.7) | 74 (76.3) | 0 | 97 | 100 (100) | 0 | 0 | 100 | 23 (23.7) | 0 (0.0) | 74 (76.3) | 0 (0.0) | 97 |
Kagera | Muleba | 8 (4.7) | 162 (95.3) | 0 | 170 | 86 (79.6) | 22 (20.4) | 0 | 108 | 4 (3.7) | 1 (0.9) | 82 (75.9) | 21 (19.4) | 108 |
Total | 107 | 821 | 0 (0) | 928 | 700 | 150 | 4 | 854 | 99 (13.2) | 6 (0.6) | 601 (70.1) | 144 (16.0) | 850 |
Discussion
Historically, pyrimethamine has been in use in Tanga region since the 1950s [
38]. In 1954 resistance to a weekly prophylactic dose of pyrimethamine was reported in Tanga and this was the first resistance report in Tanzania and in Africa [
39]. SP continued both as the second-line treatment drug [chloroquine (CQ) was the first-line drug] and for malaria prophylaxis until 2001, when it was declared the first-line drug due to high levels of CQ resistance [
40]. However, since resistance to SP had already emerged, at least in some parts of the country, SP policy in 2001 was considered a temporary solution [
41] and was replaced by ACT by 2006 [
42].
In the East African region, the prevalence of molecular markers of SP resistance has been increasing since the emergence of the first resistance-conferring mutations in the 1950s. During the past decade, many of these mutations in
Pfdhfr and
Pfdhps have approached fixation levels, while newer mutations are still increasing [
20,
27,
43,
44]. Given the importance of preventing malaria in pregnancy, the growing evidence of declining effectiveness of the IPTp strategy in areas of high prevalence of quintuple and sextuple
Pfdhfr/Pfdhps haplotypes and the lack of an alternative to SP for use in IPTp, then the monitoring of SP resistance is crucial [
45]. This is the first multi-site study in Tanzania to report on countrywide prevalence of these markers of SP resistance of immediate importance. The
Pfdhps A581G mutation was first reported at low prevalence of 1.6 and 1.2 % in Mlimba (Morogoro) and Matema (Mbeya), respectively, in 2005 [
46]. Surveys done in Tanga (Hale) in 2006 and 2007 found the mutation at prevalence of up to 54 % [
27,
47]. In this study, Tanga region represents the highest prevalence of
Pfdhps 581G followed by Kagera region. Highest levels of molecular markers of resistance (or tolerance) to other anti-malarial drugs, such as CQ, have also been recorded in Tanga when compared to other regions in Tanzania regarding mutations in
Pfcrt (reviewed in [
33]) and artemether-lumefantrine regarding the Pfmdr1 marker [
48]. Furthermore, occurrence of the South Asian CQ-resistant
Pfcrt haplotype SVMNT was also reported in Tanga for the first time [
49].
Local drug pressure is mainly related to local malaria endemicity, which meaning that resistance levels may vary between different regions in Tanzania, due to their differences in malaria endemicity. The whole of Tanzania is endemic to malaria, but the Indian Ocean coastal strip (Tanga, Coastal, Dar es Salaam, Lindi, Mtwara) and the Lake Victoria shores (Mwanza, Kagera) have generally higher malaria endemicity compared to the rest of the country. The high malaria endemicity in, especially, Tanga and Kagera may therefore partly explain the observed high resistance to SP in these regions due to increased drug pressure relative to other regions. However, the differences in levels of resistance markers between these regions compared to the Coastal region, which also represents high malaria endemicity, leads to speculation that other local factors are contributing to local expansion of the 581G mutant parasites. Such factors may be related to local movement of the population and the in- and out-flow of people carrying parasites from one area to another. For instance, according to a study by Pindolia et al. [
50], the Dodoma region is a major source of both human movement and malaria movement. Pindolia and colleagues have shown that while the majority of both human and malaria movement is directed towards the central and the western parts of the country, which do not represent major sources of super resistance (mainly Mbeya and Mwanza), the majority of the malaria movement was directed towards Mwanza (where there is some degree of resistance). This implies that the malaria movement does not correlate positively with resistance. Tanga, however, which represents the highest level of SP resistance was found to represent only internal movement and no major in- or out-flow or neither people nor malaria, indicating that perhaps this setting is more isolated and prone to resistance emergence and accumulation, perhaps due to a lack of in-flow of new and diverse parasite genotypes.
Furthermore, the southern parts of the Tanzania have a lower level of SP resistance, whereas the trends shown in the present study point to the northeastern and northwestern parts bordering Kenya and Uganda, respectively, having relatively higher levels of SP resistance. It is possible that cross-border spread of resistance contributes to these observations. For instance, in western Kenya,
Pfdhps 540E and 581G have been reported to have increased, respectively, from 33.1 and 0 % in 1996 to 99.2 and 5.3 % in 2009 [
43]. Related trends have also been reported in the same area in Kenya [
51] although the reported prevalence of 581G is much lower than in Tanga and Kagera regions. In Uganda, a study performed in central Uganda reported
Pfdhps 581G at 3.3 %, while another in western Uganda reported 36 % [
28,
52].
Considering the combined
Pfdhps K540E-A581G haplotypes, the EG haplotype (540E–581G) was observed at highest prevalence (>50 %) in Tanga region (both in Muheza and Bondo sites) and in Kagera (>20 % in Muleba). This haplotype is common in South America and Cambodia [
53] thus it unclear whether this has independently evolved in Tanzania or other factors such as importation account for this. The EA highest in Mbeya and Mwanza regions (>90 %) was considered an East African haplotype, while the rarely observed wild-type KA is common in West Africa. A rare KG haplotype in was observed in Tanga. The KG is thought to evolve from the EG haplotype and is common in Cambodia and Venezuela [
53]. The overall distribution of
Pfdhps mutation and especially the EG haplotype indicates that
P. falciparum sensitivity to SP vary largely across the country, with implication for SP-IPTp implementation. Despite the large sample set from across Tanzania used in this study, it is not clear if a greater variability can be found if further sampling is performed. Furthermore, intra-regional variability in resistance has been observed, for instance, for the case of Bondo and Muheza within Tanga region. Further preliminary mapping of the
Pfdhps K540E-A581G haplotypes using 2014 samples from Songea in Ruvuma region, which is placed somewhat between Mtwara and Mbeya, observed a prevalence of the EG haplotype of 2 % (Fig.
1), which does not differ much from the 5 % in neighbouring Mtwara region. A similar observation was made for Mwanza.
Sporadic evidence shows that although ACT is the current first-line anti-malarial for treatment of uncomplicated malaria, the lack of proper healthcare services, especially in rural communities in Tanzania, as well as the availability of other anti-malarials in drug shops, encourages self-medication with non-standard regimens, including SP [
54,
55]. It is important for national malaria control programmes and Ministries of Health to limit the availability of drugs such as SP to IPTp and/or IPTi programmes only. Furthermore, consideration for differentiated regional implementation of SP-IPTp based on differences in resistance levels may be important prior to availability of alternatives to SP. Sustained monitoring of molecular markers of SP resistance, especially super-resistance markers, should be continued with countrywide coverage in order to enable time-point specific assessment.
Authors’ contributions
RAK conceived the idea, designed the study, analysed the data, and wrote the manuscript. RDK performed laboratory work and participated in data analysis and writing the manuscript. SN participated in data interpretation and writing the manuscript. CK and JGN participated in sample collection, laboratory work and reviewed the manuscript. AAK participated in sample collection, data interpretation and reviewed the manuscript. DI participated in data analysis and revised the manuscript. CR and MA participated in overall study design, data analysis and interpretation, and in writing the manuscript. All authors read and approved the final manuscript.