Background
Malaria remains an important health problem in several countries in the world especially in Thailand [
1,
2]. Cerebral malaria is one of the major pathological complications of
Plasmodium falciparum infection in humans, manifesting as coma that can lead to death. The pathogenesis of cerebral malaria remains controversial, but major factors involved,
i.e., cytokines and adhesion molecules are well documented [
3]. In Thailand, malaria is still problematic in particular areas, especially in the forest and forest fringes along international borders where there is significant population movement. The highest cases of malaria in 2009 were reported from Tak Province, where Mae Sot District is located. They have carried the largest burden of malaria diagnosis and treatment for foreigners, the majority of whom are from Myanmar [
2]. Mae Sot District is also an endemic area polluted with high levels of cadmium [
4‐
6]. The degree of soil cadmium contamination is associated with rice grain cadmium contamination downstream of an actively mined zone of zinc mineralization in Mae Sot District [
6]. Population cadmium exposure is due mainly to eating contaminated food, smoking cigarettes, and occupation in cadmium-contaminated places [
7]. There have been several reports on the involvement of cadmium in nephropathy [
5,
7,
8].
Haem oxygenase (HO) enzyme is proposed as one of the factors that may play role in pathogenesis including susceptibility and severity of malaria disease [
9,
10]. The isoforms HO-1 and HO-2, are microsomal enzymes that play important role in haem catabolism to produce biliverdin/bilirubin, carbonmonoxide and iron [
9,
11‐
13]. The promoter region of HO-1 gene contains cadmium response element (CdRE), the binding site for cadmium which is a potent inducer of HO-1 transcription [
14]. Therefore, it may be possible that the linkage of cadmium exposure and susceptibility to malaria disease is through binding of cadmium to CdRE of the HO-1 gene. The polymorphism of human HO-1 gene promoter compose of the single nucleotide polymorphism (SNPs) and (GT)
n dinucleotide polymorphism which may contribute to the fine tuning of the transcription. Long (GT)
n alleles have been found associated with susceptibility to smoking-induced emphysema or coronary artery disease, while they may be linked to resistance to cerebral malaria [
10,
15,
16].
TNF is a cytokine produced primarily by monocytes and macrophages in many inflammatory diseases. SNPs of the TNF promoter have been reported to be associated with susceptibility to severe malaria. Four mutations are transitions of adenosine to guanine and are located at nucleotide positions -238, -244, -308, and -376, relative to the transcriptional site [
17,
18]. Various studies have investigated the relation existing between TNF promoter alleles and severity of malaria. TNF has been shown to be elevated in severe malaria [
19], and TNF promoter region -238A allele together with -376A allele are associated with susceptibility to severe malaria [
20,
21]. Furthermore, TNF P-D allele has been shown significantly associated with cerebral malaria in our previous study in Karen and Burmese populations [
22].
In this study, the (GT)n repeat polymorphism in the promoter region of the inducible HO-1 and six mutations of TNF from malaria patients (Thai, Burmese and Karen), in Mae Sot endemic area, were analysed. The aim was to determine the association between genetic polymorphisms of HO-1, TNF and severity of malaria infection.
Discussion
The association between human haem oxygenase-1 (HO-1) and pathogenicity/severity of malaria infection was described in a few studies
in vitro including molecular epidemiological investigation from brain lesion [
24,
29,
30] and the hypothetical roles of HO-1 in pathogenesis of cerebral malaria was proposed by Shibahara [
10]. However, only one research article which provides evidence on the association between (GT)
n repeat polymorphism of HO-1 and malaria pathogenicity/severity was reported in Karen ethnic minority group with cerebral malaria and acute uncomplicated falciparum malaria who resided in areas along the Thai-Myanmar border [
24]. In that study, the proportion of patients with short (GT)
n alleles was found to be significantly higher in cerebral malaria (SM) than UM. Short (GT)
n alleles in the promoter region may therefore represent a genetic risk factor for cerebral malaria as in may directly enhance the transcription of HO-1 in malaria patients, and as a consequence, the products of haem degradation,
i.e., CO, iron and bilirubin, may increase in the brain lesion. Furthermore, the influence of the (GT)
n repeat polymorphisms in the HO-1 gene promoter was investigated in different cell lines where constructs with lengths of less than 25 repeats (short repeat) showed an increasing HO-1 basal promoter activity [
31] or transcriptional up-regulation in response to various stimuli as compared to that with greater than 25 repeats [
15]. Increasing transcriptional up-regulation leads to high activity of HO-1 enzyme and thus, the haem degradation products particularly iron, which is an essential supply for growth and proliferation of malaria parasite. Excess amount of iron might trigger high parasitaemia causing red blood cell haemolysis and severe malaria including cerebral malaria.
The present study, due to limitation of available data on (GT)
n repeat polymorphism of HO-1 in different patient populations with different malaria severity, estimation of proper sample size was not possible. There appears to be a significant difference in HO-1 genotypes among the three ethnics. This may explain difference in pathogenicity/severity of malaria infection in various ethnics. The frequencies of short (GT)
n alleles (S/S) genotype in the three groups of patients with different disease severity (combined ethnics) were found to be comparable. This lack of association could represent a genuine finding, or else, a low study power due to inadequate sample size (particularly in the SM group). In addition, the major confounding factor ethnics cannot be excluded. In a previous study, a significant association between the short (GT)
n alleles (S/S) polymorphism of HO-1 gene promoter and increased risk of cerebral malaria (severe malaria) has been demonstrated in 150 Burmese and Karen patients [
24]. Nevertheless, the sample size included in that study was unbalanced and also too small (30 cases of cerebral malaria, 120 cases of UM) to provide a definitive conclusion on such association. The finding of the lack of association between genetic polymorphism of HO-1 (GT)
n repeat and malaria disease pathogenicity/severity found in this study may not entirely exclude the possible link between HO-1 enzyme activity and malaria disease pathogenicity/severity. Results from recent
in vitro study provide insight into the molecular mechanism of induction of HO-1 activity and the link with malaria pathogenicity/severity [
10,
24]. Treatment of astrocyte (CCF-STTG1) and retinal pigment epithelial (ARPE-19, D407) cells with exogenous prostaglandin D
2 (PGD
2) and 15d-PGJ
2 (metabolite of PGD
2) consistently induced the expression of HO-1 mRNA and protein [
32,
33]. PGD
2 is a major prostanoid produced in the brain and is involved in the regulation of sleep and pain responses [
34].
Cadmium has been shown to be a potent inducer of HO-1 activity [
14,
35], and as a consequence, this might be linked to severity of malaria disease. Blood cadmium reflects recent cadmium exposure, whereas urinary cadmium indicates body accumulation of cadmium [
7,
36]. The ratio of plasma to blood cadmium varies from 3 to 16% [
37]. The observed median (range) values of plasma cadmium concentrations in the VM, UM and SM groups of patients were 0.10 (0.01-0.33), 0.24 (0.01-3.18) and 0.16 (0.03-2.34) μg/L, respectively. Twenty-one patients (in SM and UM groups) had the concentrations above the tolerance limit of 0.5 μg/L [
38]. The information on blood cadmium concentrations in Thai population has been reported in non-occupational females living in Bangkok and other areas, with the geometric mean blood levels of 0.40 and 0.43 μg/L, respectively [
39]. The observed concentrations of cadmium in plasma in malaria patients were considered higher than non-occupational residents in other areas due to the fact that cadmium level in plasma is only about 3-16% of that in blood [
40]. Although the concentrations of plasma cadmium are still considered low considering the threshold level of 0.5 mg/L, results may more or less explain the high incidence of malaria case report, mortality and morbidity from this high cadmium pollutant area of Mae Sot. It appears that plasma cadmium concentrations tended to be higher in patients with falciparum malaria (UM and SM) compared with VM. In addition, significantly lower proportions of cases with falciparum malaria including both UM (80.4%) and SM (76.9%) were found compared with VM (100%) at plasma cadmium level of ≤ 0.5 μg/L. Cadmium is known to produce toxic effect to human and other organisms including malaria parasite when exposing with high level of cadmium. It is possible that optimally high levels of cadmium might promote the growth of
P. falciparum but not with
P. vivax by inducing HO-1 activity to produce iron. The mechanism(s) by which parasite transport or demolish cadmium are, therefore, important for their survival. It has been reported that
P. falciparum efflux cadmium from cells through PFMDR2 protein [
41]. Again, due to limited sample size and confounding factors (age, gender, ethnic), definitive conclusion on this association could not be obtained. Cadmium concentrations have been reported to vary markedly according to age, gender and ethnic [
42,
43] and results from the present study also revealed some association between ethnicity (Thai
vs Burmese) and cadmium levels in group with level of ≤ 0.5 μg/L.
Several articles have reported the involvement of cytokines in the histopathology of cerebral malaria [
44,
45]. Among these cytokines, TNF is thought to play a major role in pathogenesis of cerebral malaria. Others have reported the presence of cytokines in the brain after fatal cases of malaria [
45,
46]. Three SNPs of TNF promoter -857, -863 and -1031 were analyzed and the frequency of the designated allele -857C/-863C/-1031C was found to be significantly higher in patients with cerebral malaria than that with UM in area along Thai-Myanmar border [
28]. In the present study, the frequency of -857C/-863C/-1031C was found to be 1.3, 4.0 and 3.1% in Thai, Burmese and Karen patients, respectively. It was noted however for the observed lack of significant difference in frequency of this promoter allele (-857C/-863C/-1031C) between the SM and UM groups. The TNF polymorphism was categorized based on the patterns of allele polymorphisms reported by Ubalee [
22] and Hananantachai [
28]. The first classification-- TNF P-A, TNF P-B, TNF P-C, TNF P-D, TNF P-E and TNF P-F was based on the biallelic polymorphism sites at nucleotides -238, -308, -857, -863 and -1031. The second classification-- TNF P1, TNF P-2, TNF P-3, TNF P-4 and TNF P-5 was based on the biallelic polymorphism sites at nucleotides -857, -863 and -1031. No significant association between any pattern of TNF polymorphism as well as each individual single SNPs and disease pathogenicity/severity (SM, UM, VM) including ethnics (Thai, Karen, Burmese) were observed when polymorphisms were classified based on both criteria. The biallelic polymorphic sites at nucleotides -238, -308, -857, -863 and -1031, with seven allele patterns (TNF P-A, TNF P-B, TNF P-C, TNF P-D, TNF P-M1, TNF P-M4 and TNF P-M7) were identified in a previous study in Burmese and Karen patients who lived near Thai-Myanmar border [
22] and TNF P-D allele was found to be significantly associated with the high proportion of cerebral malaria (SM) compared with UM cases. Interestingly, the TNF P-M1, TNF P-M4 and TNF P-M7 but TNF P-E and TNF P-F were not found in all the three ethnics under the present investigation. The frequencies of the -863C or -1031T allele, the typical polymorphisms of TNF P-D, were found much higher in Swedish (94% for -863C and 80% for -1031T) [
47] and in Japanese (82% for -863C and 84% for -1031T) subjects [
25] than in the three ethnics under present investigation where the frequencies of -863C and -1031T alleles were 38
vs 39% in Thai, 40
vs 38% in Burmese and 41
vs 40% in Karen patients, respectively. The association of single SNP of TNF was also found in other studies in African patients. Two studies were performed in Gambian children and results showed that the TNF -238 A allele was found to be associated with susceptibility to severe malarial anaemia but not to CM [
20]. On the other hand, the neighbouring TNF -308 A allele was associated with CM but not with severe malarial anaemia [
48]. Furthermore, data from 1,048 Kenyan children showed the TNF -308 A allele to be significantly associated with high density
P. falciparum parasitaemia. Among low birth weight children, the TNF -308 A allele was also found to be associated with severe anaemia with a trend toward a risk for severe malaria anaemia [
49]. In contrast with other studies, a study conducted in Gabon comparing malaria severity and TNF promoter (TNF P) variants has demonstrated that the frequencies of carriers of distinct TNF variants did not differ significantly in the groups with mild and SM [
18]. Moreover, TNF plasma levels were not significantly associated with any of the TNF variants.
Competing interests
The authors declare that they have no competing interests.
Authors' contributions
JK performed the molecular genetic studies, participated in the sequence alignment, interpretation of data, performed the statistical analysis and drafted the manuscript. KH participated in the design of the study. MK participated in the molecular genetic studies and sequence alignment. RR participated in sample collection and the study design and coordination. KN participated in the design of the study, performed the statistical analysis and finalised the manuscript. All authors read and approved the final manuscript.