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Human Genetic Markers and Structural Prediction of Plasmodium falciparum Multidrug Resistance Gene (pfmdr1) for Ligand Binding in Pregnant Women Attending General Hospital Minna.

1. Introduction

Malaria is a vector borne infectious disease endemic in Nigeria with about 97% of the population at risk [1]. In Nigeria, malaria accounts for 60% of outpatient visits to health facilities, 25% of childhood death, and 11% of maternal death [2]. The financial loss due to malaria annually is estimated to be about 132 billion naira in form of treatment cost, prevention, and loss of man hours, among others [3]. Increased resistance of the Plasmodium falciparum parasite to many of the available antimalarial drugs has made the treatment of malaria increasingly difficult and poses a major threat to the malaria control and eradication program running across the globe [4]. The factors influencing the rate of spread of antimalarial drug resistance include de novo mutation, human population movement and infection among migrants, drug use, and malaria transmission intensity [5]. More than any other issue, poverty, in adherence to drug prescription, and inadequate access to drugs continue to be major force in the development of resistance. A wide range of unrecommended antimalarial medicines are available and sold over the counter in medicine stores and are accessible to multigravid pregnant women in Nigeria [1]. Healthcare providers also prescribed unrecommended antimalarials due to poor knowledge on best practices and low confidence in the recommended drugs. The impact of antimalarial drug resistance includes high mortality (resistant infections are more often fatal) and morbidity. Resistance to antimalarial drugs has also increased the global cost of controlling the disease and investigations on newer and more expensive drugs. Therapeutic failure necessitates consultation at a health facility for further diagnosis and treatment, resulting in loss of working days for adults and absence from school for children.

Malaria during pregnancy is a major public health concern. In most endemic areas, pregnant women are the main adult risk group for malaria [6]. Pregnant women are particularly susceptible to severe malaria and have a greater risk of antimalaria resistance due to loss of immunity during pregnancy, thus placing them at high risk of maternal and infant morbidity and mortality, abortion, premature labour, and stillbirth [7].

Genetic markers such as hemoglobin genotypes and blood groups have been associated with malaria but have been implicated with rosette formation and cytoadhesion [8]. Variations in gene encoding functional glycotransferase have been associated with protection from P. falciparum malaria. Also trisaccharide of "A" and "B" blood group is presumed to act as receptor and function as an important factor for rosetting. However, the RBC of group O does not express trisaccharide blood types [9].

Genetic variations in pfmdr1 gene have played vital role in malaria chemotherapy. Mutations (N86Y, Y184F, S1034C, N1042D, and D1246Y) in the pfmdr1 gene have been associated with resistance to multiple antimalarial drugs such as quinine, mefloquine, halofantrine, artemisinin, lumefantrine, CQ, and amodiaquine [10-13]. However, mutations in this gene have been associated with geographic areas [14], and there is a paucity of information on antimalarial drug resistance markers in Plasmodium falciparum infected pregnant women in Northern Nigeria. Therefore, it becomes relevant to determine the molecular marker of resistance in populace of this region. Also, understanding the relationship between pfmdr1 amino acid sequence and its three-dimensional structures will assist in predicting the chemical ligands/inhibitor that can bind and change the functional integrity of the proteins. This will provide information that is crucial in designing an alternative and effective antimalarial drug, thus providing a new window for malaria drug target.

2. Materials and Methods

2.1. Study Area. This study was carried out in Minna, Niger State located in the tropical zone of North Central Nigeria. Minna, the capital of Niger State, Nigeria, is located within longitude 6[degrees]33,E and latitude 9[degrees]377N, covering a land area of 88 [km.sup.2] with a population of 1.2 million (2006 Population Census). Minna has a tropical climate with mean annual temperature, relative humidity, and rainfall of 30.20[degrees], 61.00%, and 1334.00 cm, respectively. The climate presents two distinct seasons: a rainy season (April-October) and dry season (November-March).

2.2. Inclusion and Exclusion Criteria. All women enrolled had earlier received intermittent preventive treatments (IPTp) with sulphadoxine-pyrimethamine (SP), as per current practice. The eligibility factor was set as women presenting with gestational age 4 weeks and above to ensure adequate coverage and data control. Those who were not resident in the study area, visitors, and temporary residents who were not officially registered for antenatal were not eligible for enrolment. Other exclusion criteria included history of adverse drug reaction or severe disease (such as hepatitis, jaundice, tuberculosis, and obvious AIDS symptoms).

2.3. Ethical Considerations. This study was approved by the Ethical Committee of the Niger State Ministry of Health, Minna, Nigeria. Oral consent was obtained from the participant prior to inclusion in the study and before sample collection. All procedures were performed according to the guidelines for human experimentations in clinical research as stated by the Federal Ministry of Health of Nigeria.

2.4. Experimental Subjects and Sample Collection. A total of 250 women that attended antenatal care during the period of study (December 2016) were recruited. Each pregnant woman was finger pricked using a sterile lancet to obtain capillary blood for a rapid diagnostic test (RDT) for malaria. Safety procedures were adopted in the collection of finger-prick blood samples by swabbing the area to be sampled with 70% alcohol and allowing it to dry before collection. Two milliliters (2mL) of blood was then drawn (venipuncture) from malaria positive sample with a sterile disposable.

2.5. Parasite Detection. RDT based P. falciparum specific histidine-rich protein-2 (Bioline, USA) was performed according to the manufacturer's instructions to detect parasites as recommended by the National Malaria Programme [15].

2.6. ABO Blood Grouping and Hemoglobin Genotyping. The ABO blood group of each subject was determined using cell grouping antisera (A, B, and D) as described by Simon-Oke et al., [16], while the hemoglobin genotype separation was carried out using cellulose acetate electrophoresis method as described by Cheesbrough, [17].

2.7. Hematological Parameters. The hematological parameters, hemoglobin (Hb), Packed Cell Volume (PCV), Red Blood Cells (RBC), White Blood Cells (WBC), and platelets count (PLT), were determined using the automated hematologic analyzer SYSMEX KX21, a product of SYSMEX Corporation, Japan, as described by Dacie and Lewis, [18].

2.8. Molecular Studies

2.8.1. DNA Extraction. The genomic DNA was extracted from 2 ml of infected blood using QIAmp DNA Mini Kit (Qiagen, Hilden, Germany) according to the manufacturer's instructions and subsequently stored at -20[degrees]C until use. The presence of DNA was ascertained by subjecting it to 1% agarose gel electrophoresis (DNA GelRed[TM]) and the purity of DNA was checked spectrophotometrically by calculating the A260/A280 ratio.

2.8.2. Amplification of pfmdr1 Gene. Amplification of the pfmdr1 gene was performed on two fragments using polymerase chain reaction (PCR): the first fragment contained codons 86 and 184; the second fragment contained codons 1034 and 1042. The primers were designed on the basis of the Plasmodium falciparum 3D7 multidrug resistance protein (pfmdr1), partial mRNA sequence (GenBank accession no. XM_001351751.1). The reaction primers and conditions for amplification of the first fragment (580 bp) were Forward: AGGTTGAAAAAGAGTTGAAC and Reverse: ATGACACCACAAACATAAAT; reaction conditions were 94[degrees]C for 3 minutes/[94[degrees]C for 30 seconds, 45[degrees]C for 1 minute, 72[degrees]C for 1 minute] x 30 cycles/72[degrees]C for 5 minutes. The reaction primers and conditions for amplification of the second fragment (234 bp) were Forward: GCATTT TATAATATGCATACTG and Reverse: GGATTTCATAAAGTCATCAAC; reaction conditions were 94[degrees]C for 3 minutes/[94[degrees]C for 30 seconds, 55[degrees]C for 1 minute/65[degrees]C for 40 seconds] x 30 cycles/65[degrees]C for 5 minutes/15[degrees]C for 5 minutes [1, 13].

The PCR amplification reactions were performed in a 20pl volume PCR tube containing 1.0 U of Taq DNA polymerase (Pyro Hot Start), 250 [micro]M each of the dNTPs, 1x reaction buffer with 1.5 mM Mg[Cl.sub.2], 1x stabilizer and tracking dye, and 4 pl of genomic DNA. All PCR reactions were carried out in a thermal cycler (Techne TM Thermal cycler TC-312, Fisher Scientific, UK). PCR products were separated on a 1.5% agarose gel (Invitrogen) and stained with ethidium bromide for confirmation of amplification of the two pfmdr1 fragments as indicated by a band at 580 bp and 234 bp.

2.8.3. Sequencing Protocol for pfmdr1. Polymorphisms in the pfmdr1 gene were determined by direct sequencing of the amplicons resulting from the nested PCR using each primer for target gene amplification. The sequencing was done using BigDye Terminator v3.1 cycle sequencing kit in an ABI 3730 sequencer (Applied Biosystems). The deduced amino acid sequences were aligned and analyzed with the [Lasergene.sup.5] software (DNASTaR, Madison, WI, USA) using the reference sequences of 3D7 retrieved from Plasmodium database (

2.9. Bioinformatics Studies

2.9.1. Database Search. The similarities in sequenced PFMDR gene were compared using pairwise alignment tools ( and the nucleotides sequence was transcribed using sequence translation Transeq (EMBOSS) ( This was compared with databased sequences using basic local alignment search tools (BLASTP) search default setting ( Five hits were selected for multiple sequences alignment using Clustal Omega method BLOSUM matrix ( Specific features such as protein family, domain, cellular component, biological process, and molecular function was predicted using InterPro (

2.9.2. Receptor Protein Selection. The PDBSum (http://www and SAS databases were searched using IPFMDR sequence to download the similar protein sequence for structural prediction. The best three hits were subjected to multiple sequence alignment ( (Laskowski, 2001). The selected structure exists in chains. The chains A were retrieved from for the clustering and helical shapes alignment using ESPipt 3.0. Advanced and all the hits proteins were model PyMOL (

2.10. Statistical Analysis. Data generated from this study were analyzed using statistical package for social science (SPSS) version 16 and presented as means [+ or -] SE of the mean. Comparisons between different patient groups were carried out by t-test. The level of significance was set at p < 0.05.

3. Results

3.1. ABO Blood Groups and Genotype Distributions. Out of 250 pregnant women that were screened for malaria, 39 (15.60%) were found to be infected with Plasmodium parasites as determined by RDT. The prevalence of malaria was highest among third trimester (46.15%) as compared with the first (30.76%) and second trimester (23.07%) groups (Table 1). These differences were observed to be statistically significant (p = 0.039). All pregnant women that were positive for malaria were also tested for ABO blood (Table 2) groups and genotype (Table 3). The prevalence was higher among genotype AA (64.10%) than AS (35.89%) and this difference was not statistically significant (p = 0.206). The distribution of ABO phenotypes among malaria infection was observed not to be statistically significant (p = 0.09). The highest proportion was among individuals with O blood group (53.84%), followed by those with blood group B (25.64%), A (17.24%), and AB (7.69%)

3.2. Hematological Parameters. The levels of PCV, RBC, HGB, TWBC, and PLC in malaria infected and noninfected pregnant women attending General Hospital Minna are shown in Table 4. Test of significance (paired sample f-test) showed a significant differences in PCV and platelet count between malaria positive and malaria negative pregnant women (p < 0.05). The p value = 0.0243 and 0.007 for PCV and platelet count indicating a very significant decrease among malaria infected pregnant women.

3.3. Prevalence of Drug Resistant Molecular Markers. The genomic DNA of the 39 blood samples from malarial infected pregnant women were successfully isolated. However, out of the 39 genomic DNA samples, only 16 samples from infected women with resistance malaria were genotype for pfmdr1 gene by PCR and nested PCR, out of which 12 (75%) were successful while 4 (25%) failed. Thus pregnant women with antimalarial resistance had pfmdr1 gene prevalence of 75%. Amplification of the pfmdr1 gene was performed in two different fragments. Seven (7) samples were successfully amplified in the first fragment (580 bp) containing codons 86 and 184; six (6) samples were amplified from second fragment (234 bp) containing codons 1034 and 1042.

3.4. pfmdr1 Gene Sequence Data. No mutation was observed at codon positions 86,184,1034, and 1042 of pfmdr1 in any of the P. falciparum isolates. However, two of the isolates from the second fragment (sequence for 1034 and 1042) showed disrupted protein sequence (Table 5)

3.5. Bioinformatics Database Search. The amino acids and translated protein sequence of the of pfmdr1 gene isolated from pregnant women attending General Hospital Minna are shown in Table 6. Although pairwise alignment of these two genes shows high (88%) percentage similarities and 3% gap between the sequences (Figure 5), BLASTP search of the second gene showed no significant similarity; however, the first gene produced multiple hits, out of which five (5) hits were selected for multiple sequence alignment. The results show very high similarities of the gene with those reported from other African countries (Figure 1).

3.6. Receptor Protein Selection. The PDBSum search of IPFMDR sequence retrieves seven (7) hits of similar protein sequence for structural prediction (Table 7). However, 4RHS, SPLTB, STT, and 5LUQ are the most similar protein with 31.7 and 34.8 percentages.

T-Coffee and ESPript 3.0 show multiple sequences alignment of pfmdr1 homologous protein of crystal structure of an inward-facing eukaryotic ABC multidrug transporter (IEMDT), crystal structure of pltb (SPLTB), and structure of typhoid toxin (STT). The T-Coffee alignment shows percentage similarity of homologous protein IEMDT, SPLTB, and STT to be 37, 64, and 65, respectively (Figure 2), while ESPript 3.0 shows the 3-dimensional helical folding of the homologous protein (Figure 3). IEMDT has twenty-one [alpha]-helices, twelve [beta] strands, and two n, while SPLTB and STT have two [alpha]-helices and five [beta] strands (Figure 4).

4. Discussion

Pregnant women living in malaria endemic regions, particularly in sub-Saharan Africa are associated with a high frequency and density of Plasmodium falciparum parasite with high rates of maternal morbidity [19]. The prevalence of malaria demonstrated in this study was 15.60% lower than 52% and 88.2% reported among pregnant women attending antenatal clinic in southwest Nigeria [20, 21].

Previously, the reports of the prevalence of malaria in pregnancy were variable and high in Niger State where prevalence rates between 58.2% and 83.40% were documented [22, 23]. High prevalence of malaria in pregnancy (41%) has been attributed to poor compliance to the use of insecticide treated nets and intermittent preventive therapy [24]. However, these reports contrast sharply with the findings of this study where a prevalence rate of 15.60% was obtained for the pregnant women attending General Hospital Minna. This finding is not surprising as all women enrolled in this study had earlier received IPTp with SP, as per current practice in Niger State. Previous researchers have also shown strong correlation between the use of long lasting insecticide treated nets (LLIN) and reduction in prevalence of parasitaemia and anaemia in pregnant women, stillbirths, and improvements in birth weights of babies [25, 26]. Thus the low prevalence rate recorded in this study may be attributed to the improved understanding and compliances of the antenatal clinic women about malaria control strategies like use of LLIN and/or alternative intermittent preventive treatment with pyrimethamine sulfadoxine (SP). In addition, the lower prevalence obtained in this study might be due to the fact that this study was carried out during the dried season as opposed to the works of Omalu et al., [22], and Ejima et al., [23], that were carried out during raining season. This finding agrees with Ayanda [27], who opined that prevalence of P. falciparum infection is higher in the wet season than in the dry season, while Minakaw et al., [28], reported that rainy season presents favorable environmental conditions that enhance mosquito breeding and survival, through the proliferation of larval habitats and improved humidity, respectively.

Various researchers have reported high seroprevalence of malaria at different trimesters of pregnancy [29]. However, according to gestational age of pregnancy, this study recorded the highest seroprevalence rate in the third trimester followed by the first trimester and least was recorded among subjects in their second trimester. This finding agrees with the works of Idowu et al., [29], Ejima et al., [23], and Omalu et al., [22], which recorded high seroprevalence in third trimester and least in second trimester, but does not correlate with the work of Brabin, [30], who reported higher prevalence in the second trimester of pregnancy, while Allesandro and Langerock, [31], and Obianumba, [32], identified higher risk of malaria in the first trimester of pregnancy. However, the 3rd trimester being of highest seroprevalence rate of malaria infection as obtained in this study suggests that the pregnant women have significant loss of immunity during late pregnancy.

The notion of pregnancy as an altered state of immune suppression is well documented [33, 34]. Third trimester of pregnancy is a time period that poses a risk of increased susceptibility to parasitic and infectious diseases, since the maternal immune system is solely responsible for defending against infections and protecting the fetus because both the fetal and the placental responses are limited [35]. This may have been the reason for the higher susceptibility to malaria by women in their third trimester of pregnancy, as recorded in this study

Therefore, the pregnant women in this area may have evidence of malarial infection at the time of birth if proper control and preventive measures are not taken, thus increasing the susceptibility of their offspring to incidence of congenital malaria, low birth weight, and mortality. In support of this claim, Omalu et al., [36], reported 2.63% congenital malaria, 4.61% placental malaria, and 5.92% cord malaria with low birth weight but no mortality in this region (Minna, Niger State). Similarly, 5.10% prevalence of congenital malaria was recorded at Ibadan University College Hospital [37]., 46.70% at Ile-Ife, Southwestern Nigeria [38], and 13.00% at Calabar Teaching Hospital [39]. Also, the observation with second trimester could be a result of constant intermittent preventive treatments in pregnancy (IPTp) given to pregnant women during antenatal care visit which usually commence during second trimester [32]

Rapid diagnostic test (RDT) has been recommended to improve diagnostic efficiency, which is important for preventing indiscriminate use of ACT, thereby preventing or delaying the development of parasite resistance to this new first-line drug [40]. Also, RDTs can be used as a stop-gap when microscopy services are not operating or as a primary diagnostic tool for rural/remote areas without microscopy services [41]. The sensitivity of RDT reported in this study (75%) is lower than 100% sensitivity previously reported in Nigeria [42] and 96%, 97%, and 97.6% reported in Zambia, Zanzibar, and Thailand, respectively [40, 43, 44]. However, percentage of patients that were false positive (25%) recorded in this study is considerably high. This suggests that there were chances of RDT to classify a healthy patient as being sick. Ayogu, [45], reported a very low (3.2%) failure of PCR confirmation of malarial patient who tested positive by RDT. The patients with false positive result by RDT are likely to be patients with persistently circulating antigen due to prior use of antimalarial. However, other factors not investigated in this work, such as age differences in sensitivity to RDT, rheumatoid factor cross-reacting in the blood [46], and cross-reactivity with heterophile antibodies [47], can be responsible for false positive result in RDT. It is therefore necessary to consider clinical situations and laboratory and especially microscopic confirmation tests in cases of suspected false positive results for malaria RDT [48].

Prevalence of malaria parasites seemed to be relatively high across a blood group O (53.84%) and AB (7.69%) subjects recording the least infection rates. High prevalence of infection in blood group O shows that they are most susceptible to uncomplicated malaria infection. This disagrees with the findings of Simon-Oke et al., [16], who reported that prevalence of malaria parasites was highest among those with AB blood group (60.0%) and lowest in those with B blood group (37.2%).

Natural selection for resistance against malaria may favor blood group O as it protects against severe P falciparum malaria [49]. However, it should be clear that the high occurrence of malaria in blood group O in this study population is not surprising, as the finding does not disapprove the hypothesis about a selective survival evolutionary advantage of P. falciparum infection in blood group O compared with non-O blood groups in malaria endemic areas, but rather further explains the hypothesis that O blood type groups are more susceptible to uncomplicated malaria but less susceptible to complicated malaria. This corresponds to the result of Rowe et al. [8] in Mali, where blood group O had a higher prevalence of uncomplicated malaria.

There are numerous publications on the strong protection of the HbAS trait against mild and severe falciparum malaria. However, this study shows that pregnant women with genotype "AA" were most susceptible to malaria with 64.10% of the total infection compared to AS (35.89%). These are not surprising, as similar occurrences have been reported in other parts of Nigeria and other African countries [5056]. It has been recorded by Friedman, [57], that the lowering of oxygen which causes sickling shape in the blood of SS and AS people reduces the parasite growth and can cause the parasites to die, but this is not so with the AA genotype. Genotype AA is the most prevalent genotype in this part of the world and more prone to malaria infection than other genotypes because of the absence of any sickle cell molecules in the blood.

Anaemia in falciparum malaria is mainly due to the destruction of parasitized red cells. However, according to Ogbodo et al., [58], increased parasite density ultimately leads to increase in red cell breakdown and consequently anaemia. Brabin, [30] reported 70-80% of pregnant women in malaria area are susceptible to anaemia. However, based on the definition of anaemia in pregnancy, which is PCV of less than 30% [59], infected women in this study cannot be classified as being anaemic (as the mean PCV was >30%). These findings corroborate with those of similar studies which reported PCV level of 30.16% [+ or -]5.55% [60] and 33.56 [+ or -] 0.48% [61] in pregnant women. However, the mean PCV, RBC, and HGB among malaria infected mothers were lower than mean PCV, RBC, and HGB of those without malaria parasite, which can be suggestive of vulnerability to anaemia in pregnancy, thus placing them at higher risk of morbidities such as congestive heart failure, fetal demise, and mortality associated with hemorrhage at the time of delivery [62].

The use of advanced molecular techniques is extremely useful for the detection of drug resistance in malarial parasites and plays an immense role in the epidemiological survey as well as in regular updating of the antimalarial drug policy regimes [4]. Therefore, it plays an important role in hospital-based prevalence study to monitor the drug resistance. Its use in detection of the point mutation in the pfmdr1 gene in this study reports no mutation detection at codon positions 86, 184, 1034, and 1042 of pfmdr1 in P. falciparum isolates from pregnant women in Minna, Niger State, Northern Nigeria, suggesting that these alleles are not a marker for multidrug resistant Plasmodium falciparum in Niger State, Nigeria, but larger sample size should conducted.

Plasmodium falciparum multidrug resistance gene 1 (pfmdr1) is an adenosine triphosphate-binding cassette protein located on the parasite's food vacuole and thus facilitates transport of solutes into the cell. In sensitivity to antimalarial drugs pfmdr1 acts as an active drug transporter, thus quinine and possibly other antimalarial drugs occupy the common drug binding site of pfmdr1, thereby inhibiting transport of other solutes. Mutations in this gene are known to alter the binding of this drug, thereby allowing the flow of solute via parasite's food vacuole, and thus drug resistance developed [63]. Therefore, the prediction of the structure pfmdr1 gene is important for identification of an analogous compound which can appropriately fit into the parasite food vacuole and block the flow/movement of solute into the parasite, thereby suggesting new ligand for drug target modification.

Basic local alignment search tool (BLAST) is the tool most frequently used for calculating sequence similarity [64]. The table of BLAST hits is a section showing all of the alignment blocks for each BLAST hit. The sequence alignments show us how well the pfmdr1 gene isolated matches pfmdr1 gene reported in the database for other African countries. It has been reported that BLAST results with sequence identity ranges of 75-92% have high degree of sequence homology [65]. In this study, it was noted that the five hits match much better the query pfmdr1 sequence than the remaining BLAST hits, and the MSA of these genes shows very high similarities of the gene with those reported from other African countries, therefore suggesting that a particular ligand could be predicted to target pfmdr1 gene in P. falciparum there by opening a novel window for malaria drug discovery.

It has been reported that molecular interaction and function of a protein depend on its three-dimensional structure [64]. Thus, prediction of protein structures assists in predicting the chemical ligands/inhibitor that can bind and change the expression or inhibit its expression, thus providing a new window for drug target.

On the basis of this, pfmdr1 gene was searched for similar protein sequence (homologous protein sequence) and structure prediction through PDBSum databases. However, 4RHS, SPLTB, STT, and 5LUQ are the most similar proteins with 31.7 and 34.8 percentages. T-Coffee and ESPript 3.0 show that there is a good alignment and orientation of pfmdr1 gene sequence with crystal structure of pltb (SPLTB) and structure of typhoid toxin (STT). This suggested that this gene shares structural identity.

T-Coffee has been reported to be definitely superior to other MSA programs with regard to alignment accuracy in all datasets [66]. Its alignment similarities ranges of 58%-91% have been considered to be of high degree [67]. In this study, alignment of pfmdr1 shows a high degree of homology to the STT (65%) and SPLTB (64%). IEMDT, however, shows least similarities of 37% (Figure 2). In the 3-dimensional helical folding of the homologous proteins, IEMDT shows twenty-one [alpha]-helices, twelve [beta] strands, and two n, while SPLTB and STT have two [alpha]-helices and five [beta] strands (Figure 3). This further removes IEMDT as a strong structural prediction for in pfmdr1.

However, it has been reported that typhoid toxin (STT) exhibits strong selectivity for Neu5Ac-terminated glycans, which is predominantly expressed in human cells, over Neu5Gc-terminated glycans, predominantly expressed by most other mammals. This toxin bound a diverse group of sialylated glycans with preferential binding to termini with the consensus sequence Neu5Ac[alpha]2-3Gal[beta]1-3/[beta]1-4Glc/GlcNAc. Therefore the exquisite binding selectivity of typhoid toxin for glycans predominantly expressed in human cells provides an explanation for the inability of S. typhi to cause typhoid fever in some nonpermissive species like chimpanzees. This is consistent with previous results on crystal structure of pltb (SPLTB) and crystal structure of gd2 bound pltb which show similar structural conformation with pfmdr1 gene isolated in this study [68]. Since, crystal structure of pltb and typhoid toxin share similar structural conformation with the isolated pfmdr1 gene in this study, this could also be the reason why P. falciparum causes malaria only in humans. Conclusively, this compound (Neu5Ac[alpha]2-3Gal[beta]1-3/[beta]1-4Glc/GlcNAc) can theoretically bind and change the functional integrity of the pfmdr1 protein, thus providing a new window for drug target.

Conflicts of Interest

The authors declare that no conflicts of interest exist regarding the publication of the manuscript.


The authors would like to thank Professors Oyekanmi Nash and Mrs. Hadiza Abdulrasheed of National Biotechnology Development Agency (NABDA), Abuja, Nigeria, for the valuable support provided during the molecular study.


[1] C. O. Agomo, W. A. Oyibo, C. Sutherland, R. Hallet, and M. Oguike, "Assessment of markers of antimalarial drug resistance in plasmodium falciparum isolates from pregnant women in Lagos, Nigeria," PLoS ONE, vol. 11, no. 1, Article ID e0146908, 2016.

[2] World Health Organization, "Global technical Strategy for malaria elimination in the in endemic countries (2016-2030)," World Health Organization Malaria Report, World Health Organization, Manila, Philippines, 2016.

[3] J. Tarning, "Treatment of malaria in pregnancy," The New England Journal of Medicine, vol. 374, no. 10, pp. 981-982, 2016.

[4] H. A. Antony, S. Das, S. C. Parija, and S. Padhi, "Sequence analysis of pfcrt and pfmdr1 genes and its association with chloroquine resistance in Southeast Indian Plasmodium falciparum isolates," Genomics Data, vol. 8, pp. 85-90, 2016.

[5] B. Lawal, O. Shittu, A. Kabiru et al., "Potential antimalarials from African natural products: a review," Journal of Intercultural Ethnopharmacology, vol. 4, no. 4, p. 318, 2015.

[6] R. McGready, S. J. Lee, J. Wiladphaingern et al., "Adverse effects of falciparum and vivax malaria and the safety of antimalarial treatment in early pregnancy: a population-based study," The Lancet Infectious Diseases, vol. 12, no. 5, pp. 388-396, 2012.

[7] P. C. Bhattacharyya and M. Nayak, "Malaria in pregnancy," Medicine Update, vol. 21, pp. 475-478, 2011.

[8] J. A. Rowe, J. M. Moulds, C. I. Newbold, and L. H. Miller, "P falciparum rosetting mediated by a parasite-variant erythrocyte membrane protein and complement-receptor 1," Nature, vol. 388, no. 6639, pp. 292-295, 1997

[9] A. Barragan, P. G. Kremsner, M. Wahlgren, and J. Carlson, "Blood group 'A' antigen is a coreceptor in Plasmodium falciparum rosetting," Infection and Immunity, vol. 68, no. 5, pp. 2971-2975, 2000.

[10] F. N. Baliraine and P. J. Rosenthal, "Prolonged selection of pfmdr1 polymorphisms after treatment of falciparum malaria with artemether-lumefantrine in Uganda," The Journal of Infectious Diseases, vol. 204, no. 7, pp. 1120-1124, 2011.

[11] V. Baraka, H. Tinto, I. Valea et al., "In vivo selection of Plasmodium falciparumPfcrt and Pfmdr1 variants by artemetherlumefantrine and dihydroartemisinin-piperaquine in Burkina Faso," Antimicrobial Agents and Chemotherapy, vol. 59, no. 1, pp. 734-737, 2015.

[12] A. F. Some, Y. Y. Sere, C. Dokomajilar et al., "Selection of known Plasmodium falciparum resistance-mediating polymorphisms by artemether-lumefantrine and amodiaquine-sulfadoxine-pyrimethamine but not dihydroartemisinin-piperaquine in Burkina Faso," Antimicrobial Agents and Chemotherapy, vol. 54, no. 5, pp. 1949-1954, 2010.

[13] G. S. Humphreys, I. Merinopoulos, J. Ahmed et al., "Amodiaquine and artemether-lumefantrine select distinct alleles of the Plasmodium falciparum mdr1 gene in Tanzanian children treated for uncomplicated malaria," Antimicrobial Agents and Chemotherapy, vol. 51, no. 3, pp. 991-997, 2007

[14] C. Fancony, D. Gamboa, Y. Sebastiao et al., "Various pfcrt and pfmdr1 genotypes of Plasmodium falciparum cocirculate with P malariae, P. ovale spp., and P. vivax in Northern Angola," Antimicrobial Agents and Chemotherapy, vol. 56, no. 10, pp. 5271-5277, 2012.

[15] Federal Ministry of Health, National Guidelines and Strategies for Malaria Prevention and Control during Pregnancy, Federal Ministry of Health, Abuja, Nigeria, 2005.

[16] I. Simon-Oke, O. Afolabi, and A. Itansanmi, "Prevalence of ABO blood groups and its relationship with malaria parasitemia among students of federal university of technology, Akure, Ondo State," International Journal of Tropical Disease & Health, vol. 17, no. 1, pp. 1-8, 2016.

[17] M. Cheesbrough, District Laboratory Practice in Tropical Countries, Cambridge University Press, Cambridge, UK, 2nd edition, 2005.

[18] J. V. Dacie and S. M. Lewis, Practical Haematology, Churchill Livinstone, London, UK, 7th edition, 1995.

[19] C. Mkandala, "The effect of malaria in pregnancy on maternal anaemia and birth weight in rural Malawi," American Journal of Tropical Medicine and Parasitology, vol. 98, no. 5, pp. 213-221, 2003.

[20] O. G. Raimi and C. P. Kanu, "The prevalence of malaria infection in pregnant women living in a suburb of Lagos," Nigeria. African Journal of Biochemistry Research, vol. 4, no. 10, pp. 243-245, 2010.

[21] O. A. Adefioye, O. A. eyeba, W. O. Hassan, and O. A. Oyeniran, "Prevalence of malaria parasite infection among pregnant women in Osogbo, Southwest, Nigeria," American-Eurasian Journal of Scientific Research, vol. 2, no. 1, pp. 43-45, 2007

[22] I. Omalu, I. Olayemi, C. Otuu et al., "Entomological and parasitological indices ofmalaria transmission in Minna, Niger State, North Central Nigeria," Advances in Research, vol. 3, no. 2, pp. 181-188, 2015.

[23] I. A. A. Ejima, M. A. Yakub, I. K. Olayemi, and S. O. Abolarmwa, "Malaria in pregnancy in minna metropolis, minna, Niger State, Nigeria," Research Journal of Medical Sciences, vol. 7, no. 4, pp. 110-117, 2013.

[24] I. Georgian, O. Matthew, and N. I. Nte, "Prevalence and effect of malaria in pregnancy among antenatal women in Ebonyi State, Nigeria," International Research Journal of Public and Environmental Health, vol. 4, no. 8, pp. 177-183, 2017

[25] C. Gamble, J. P. Ekwaru, and F. O. ter Kuile, "Insecticide-treated nets for preventing malaria in pregnancy," Cochrane Database of Systematic Reviews, vol. 19, no. 2, Article ID CD003755, 2006.

[26] T. P. Eisele, D. A. Larsen, P. A. Anglewicz et al., "Malaria prevention in pregnancy, birthweight, and neonatal mortality: a meta-analysis of 32 national cross-sectional datasets in Africa," The Lancet Infectious Diseases, vol. 12, no. 12, pp. 942-949, 2012.

[27] O. Ayanda, "Relative abundance of adult female anophelines mosquitoes in Ugah, Nasarawa State, Nigeria," Journal of Parasitology and Vector Biology, vol. 1, no. 1, pp. 005-008, 2009.

[28] N. Minakawa, G. Sonye, M. Mogi, A. Githeko, and G. Yan, "The effects of climatic factors on the distribution and abundance of malaria vectors in Kenya," Journal of Medical Entomology, vol. 39, no. 6, pp. 833-841, 2002.

[29] O. A. Idowu, C. F. Mafiana, and S. Dapo, "Malaria among pregnant women in Abeokuta, Nigeria," Tanzania Health Research Bulletin, vol. 8, no. 1, pp. 28-31, 2006.

[30] B. J. Brabin, "An analysis of malaria in pregnancy in Africa," Bulletin of the World Health Organization, vol. 61, no. 6, pp. 1005-1016, 1983.

[31] R. U. Allesandro and B. J. Langerock, "The Risks and severity of malaria in pregnant women," Applied Field Research in Malaria Reports TDR/FIELDMAL/1, WHO, Geneva, Switzerland, 1998.

[32] S. N. Obianumba, Prevalence of malaria among pregnant women attending antenatal clinic and knowledge and attitude of caregivers to malaria diagnosis In Ozubulu, Anambra State [M.S. thesis], Nnamdi Azikiwe University, 2012.

[33] A. P. Kourtis, J. S. Read, and D. J. Jamieson, "Pregnancy and infection," The New England Journal of Medicine, vol. 370, pp. 2211-2218, 2014.

[34] D. Muzzio, M. Zygmunt, and F. Jensen, "The role of pregnancy-associated hormones in the development and function of regulatory B cells," Frontiers in Endocrinology, vol. 5, article 39, 2014.

[35] G. Mor and I. Cardenas, "The immune system in pregnancy: a unique complexity," American Journal of Reproductive Immunology, vol. 63, no. 6, pp. 425-433, 2010.

[36] I. C. J. Omalu, C. Mgbemena, A. Mgbemena et al., "Prevalence of congenital malaria in Minna, North Central Nigeria," Journal of Tropical Medicine, vol. 2012, Article ID 274142, pp. 1-5, 2012.

[37] C. Falade, O. Mokuolu, H. Okafor et al., "Epidemiology of congenital malaria in Nigeria: a multi-centre study," Tropical Medicine & International Health, vol. 12, no. 11, pp. 1279-1287, 2007

[38] P. O. Obiajunwa, J. A. Owa, and O. O. Adeodu, "Prevalence of congenital malaria in Ile-Ife, Nigeria," Journal of Tropical Pediatrics, vol. 51, no. 4, pp. 219-222, 2005.

[39] A. D. Ekanem, M. U. Anah, and J. J. Udo, "The prevalence of congenital malaria among neonates with suspected sepsis in Calabar, Nigeria," Tropical Doctor, vol. 38, no. 2, pp. 73-76, 2008.

[40] M. I. Msellem, A. Martensson, G. Rotllant et al., "Influence of rapid malaria diagnostic tests on treatment and health outcome in fever patients, Zanzibar--a crossover validation study," PLoS Medicine, vol. 6, no. 4, Article ID e1000070, 2009.

[41] Ministry of Health and Medical Services, Solomon Islands 2009: Malaria Treatment Protocol, Ministry of Health and Medical Services, Honiara, Solomon Islands, 2009.

[42] O. Ajumobi, K. Sabitu, P. Nguku et al., "Performance of an HRP-2 rapid diagnostic test in nigerian children less than 5 years of age, "The American Journal of Tropical Medicine and Hygiene, vol. 92, no. 4, pp. 828-833, 2015.

[43] H. Hopkins, L. Bebell, W. Kambale, C. Dokomajilar, P. J. Rosenthal, and G. Dorsey, "Rapid diagnostic tests for malaria at sites of varying transmission intensity in Uganda," The Journal of Infectious Diseases, vol. 197, no. 4, pp. 510-518, 2008.

[44] E. Nicastri, N. Bevilacqua, M. S. Schepisi et al., "Accuracy of malaria diagnosis by microscopy, rapid diagnostic test, and PCR methods and evidence of antimalarial Overprescription in non-severe febrile patients in two Tanzanian hospitals," The American Journal of Tropical Medicine and Hygiene, vol. 80, no. 5, pp. 712-717, 2009.

[45] E. E. Ayogu, Evaluation of malaria diagnostic methods, efficacy of artemether-lumefantrine therapy and genetic determinants of Plasmodium falciparum resistance [Ph.D. thesis], University of Nigeria, 2015.

[46] M. P. Grobusch, U. Alpermann, S. Schwenke, T. Jelinek, and D. C. Warhurst, "False-positive rapid tests for malaria in patients with rheumatoid factor," The Lancet, vol. 353, no. 9149, p. 297, 1999.

[47] A. H. Moody and P. L. Chiodini, "Non-microscopic method for malaria diagnosis using OptiMAL IT, a second-generation dipstick for malaria pLDH antigen detection," British Journal of Biomedical Science, vol. 59, no. 4, pp. 228-231, 2002.

[48] J.-H. Lee, J. W. Jang, C. H. Cho et al., "False-positive results for rapid diagnostic tests for malaria in patients with rheumatoid factor," Journal of Clinical Microbiology, vol. 52, no. 10, pp. 3784-3787, 2014.

[49] Deepa, V. A. Alwar, K. Rameshkumar, and C. Ross, "ABO blood groups and malaria related clinical outcome," Journal of Vector Borne Diseases, vol. 48, no. 1, pp. 7-11, 2011.

[50] O. Kolawole, O. Ozokonkwo, and O. Mokuolu, "Prevalence of plasmodium falciparum malaria among patients attending university of Ilorin teaching hospital, Ilorin, Nigeria," Animal Research International, vol. 11, no. 3, pp. 2063-2070, 2014.

[51] S. E. Amala and C. P. Nwibani, "Malaria in children, its association with abo blood group and haemoglobin genotype," International Journal of Development Research, vol. 5, article 11, pp. 5958-5962, 2015.

[52] O. I. Leticia, O. E. Ifeanyi, C. S. Gideon, E. Queen, and O. K. Chinedum, "Determination of the haemoglobin, genotype and ABO blood group pattern of some students of Imo State University, Owerri, Nigeria," International Journal of Current Reaserch and Academic Review, vol. 3, article 1, pp. 20-27, 2015.

[53] A. J. Esan, "Assessment of haemoglobin variants in malaria infected individuals using haematological parameters," International Journal of Hematological Disorders, vol. 2, article 1, pp. 49, 2015.

[54] R. Bamou and S. L. Sevidzem, "ABO/Rhesus blood group systems and malaria prevalence among students of the University of Dschang, Cameroon," Microwave Journal, vol. 7, article 4, 2016.

[55] H. Tadesse and K. Tadesse, "Assessing the association of severe malaria infection and ABO blood groups in northwestern Ethiopia," Journal of Vector Borne Diseases, vol. 50, no. 4, pp. 292-296, 2013.

[56] E. Ito, A. Egwunyenga, and J. Ake, "Prevalence of malaria and human blood factors among patients in Ethiope East, Delta State, Nigeria," International Journal of Medicine and Biomedical Research, vol. 3, no. 3, pp. 191-201, 2014.

[57] M. J. Friedman, "Erythrocytic mechanism of sickle cell resistance to malaria," Proceedings of the National Acadamy of Sciences of the United States of America, vol. 75, no. 4, pp. 1994-1997, 1978.

[58] S. O. Ogbodo, U. I. Nwagha, A. N. C. Okaka, S. C. Ogenyi, R. O. Okoko, and T. U. Nwagha, "Malaria parasitaemia among pregnant women in a rural community Of eastern Nigeria; need for combined measures," Nigerian Journal of Physiological Sciences, vol. 24, no. 2, pp. 95-100, 2009.

[59] O. Ogunbode, "Management of anaemia in pregnancy," Nigeria Medical Practice, vol. 8, pp. 105-107, 1984.

[60] A. A. Akinbami, S. O. Ajibola, K. A. Rabiu et al., "Hematological profile of normal pregnant women in Lagos, Nigeria," International Journal of Women's Health, vol. 5, no. 1, pp. 227-232, 2013.

[61] E. A. Azab, "Haematological parameters in pregnant women attended antenatal care at sabratha teaching hospital in Northwest, Libya," American Journal of Laboratory Medicine, vol. 2, no. 4, p. 60, 2017

[62] M. Desai, F. O. ter Kuile, and F. Nosten, "Epidemiology and burden ofmalaria in pregnancy," The Lancet Infectious Diseases, vol. 7, no. 2, pp. 93-104, 2007

[63] P. E. Ferreira, G. Holmgren, M. I. Veiga, P. Uhlen, A. Kaneko, and J. P. Gil, "PfMDR1: Mechanisms of transport modulation by functional polymorphisms," PLoS ONE, vol. 6, no. 9, Article ID e23875, 2011.

[64] G. M. Boratyn, A. A. Schaffer, R. Agarwala, S. F. Altschul, D. J. Lipman, and T. L. Madden, "Domain enhanced lookup time accelerated BLAST," Biology Direct, vol. 7, article no. 12, 2012.

[65] S. F. Altschul, T. L. Madden, A. A. Schaffer et al., "Gapped BLAST and PSI-BLAST: a new generation of protein database search programs," Nucleic Acids Research, vol. 25, no. 17, pp. 3389-3402, 1997.

[66] C. Notredame, D. G. Higgins, and J. Heringa, "T-coffee: a novel method for fast and accurate multiple sequence alignment," Journal of Molecular Biology, vol. 302, no. 1, pp. 205-217, 2000.

[67] N. Schormann, B. Pal, O. Senkovich et al., "Crystal structure of Trypanosoma cruzi pteridine reductase 2 in complex with a substrate and an inhibitor," Journal of Structural Biology, vol. 152, no. 1, pp. 64-75, 2005.

[68] J. Song, X. Gao, and J. E. Galan, "Conferring virulence: structure and function of the chimeric A2B5 typhoid toxin," Nature, vol. 499, no. 7458, pp. 350-354, 2013.

B. Lawal, O. K. Shittu, A. Abubakar, and A. Y. Kabiru

Department of Biochemistry, Federal University of Technology, P.M.B. 65, Minna, Nigeria

Correspondence should be addressed to B. Lawal;

Received 15 December 2017; Revised 17 March 2018; Accepted 1 April 2018; Published 16 May 2018

Academic Editor: Francesco Pappalardo

Caption: Figure 1: Similarities of the isolated pfmdr1 gene with those reported from other African countries.

Caption: Figure 2: T-Coffee multiple sequences alignment of pfmdr1 homologous protein.

Caption: Figure 3: Clustering and helical shapes alignment of pfmdr1 gene homologous protein. Included proteins are crystal structure of an inward-facing eukaryotic ABC multidrug transporter, crystal structure of pltb, and structure of typhoid toxin. The secondary structure elements are as follows: [alpha]-helices are shown as large coils, [3.sub.10] helices are shown in small coils labeled [eta], [beta] strands are shown in arrows labeled [beta], and [beta] turns are labeled TT. The identical residues are shown on a red background with conserved residues in red and conserved regions in blue boxes.

Caption: Figure 4: PyMOL build structure of (a) STT monomers, (b) SPLTTB monomer, and (c) SPLTTB pentamer.

Caption: Figure 5: Pairwise alignment of the isolated pfmdr1 gene sequences.
Table 1: Prevalence of malaria infection among different gestation
periods of pregnant women attending General Hospital Minna.

Stages of pregnancy   Frequency (%)

1st trimester          12 (30.76)
2nd trimester           9 (23.07)
3rd trimester          18 (46.15)
t-value                  4.91
p-value                 0.039

Table 2: Prevalence of malaria infection among different blood
groups of pregnant women attending General Hospital Minna.

ABO blood groups   Frequency (%)

A                    5 (17.24)
B                   10 (25.64)
AB                   3 (7.69)
O                   21 (53.84)
t-value               2.42
p-value              0.094

Table 3: Prevalence of malaria infection among different genotype
of pregnant women attending General Hospital Minna.

Genotype   Frequency (%)

AA          25 (64.10)
AS          14 (35.89)
SS           0 (0.0)
AC           0 (0.0)
t-value      1.609
p-value      0.206

Table 4: Hematological parameters in Plasmodium falciparum infected
pregnant women attending General Hospital Minna.

Subjects                           PCV (%)             HGB (g/l)

Malaria Positive (N = 20)    33.56 [+ or -] 4.01   8.93 [+ or -] 1.09
Malaria Negative (N = 10)    44.50 [+ or -] 3.20   9.03 [+ or -] 1.47
p-value                            0.0243                0.195

Subjects                            RBC           WBC (x[10.sup.9]/L)

Malaria Positive (N = 20)    5.97 [+ or -] 0.68   4.80 [+ or -] 0.32
Malaria Negative (N = 10)    7.01 [+ or -] 1.76   4.20 [+ or -] 0.45
p-value                            0.194                 0.271

Subjects                     Platelet (x[10.sup.3]/L)

Malaria Positive (N = 20)     267.89 [+ or -] 26.90
Malaria Negative (N = 10)     598.67 [+ or -] 39.77
p-value                               0.007

Red blood cells (RBC), haemoglobin (HGB), packed cell volume (PCV),
total white blood cell (WBC), and differential counts.

Table 5: Protein sequence of Pfmdr1 gene isolates from genomic DNA of
P falciparum infected pregnant patient sample.

Sample code         Primers used                Protein sequence



Sample code   S1034C   N1042D

A1              W        W

A3              D        D

W: wild type; D: disrupted protein sequence.

Table 6: Amino acid and translated protein sequence of the pfmdr1
gene fragments.

Amino acid sequence                     Translated protein sequence



Amino acid sequence                      Blastp result



Table 7: PDBSum database information ofpfmdrl
gene homologous protein sequence. Sequence:
Sequence length: 67 residues.

                                               %-tage     a.a.
PDB code             Model           Length   identity   overlap

1 3wmg(A)    X-ray 2.40 [Angstrom]    589      27.3%       44

2 3wmf(A)    X-ray 2.60 [Angstrom]    588      27.3%       44

3 IEMDT(A)   X-ray 2.75 [Angstrom]    588      27.3%       44

4 4rhs(A)    X-ray 1.92 [Angstrom]    114      31.7%       41

5 SPLTB(A)   X-ray 2.08 [Angstrom]    114      31.7%       41

6 STT(A)     X-ray 2.39 [Angstrom]    114      31.7%       41

7 5luq(A)    X-ray 4.30 [Angstrom]    3725     34.8%       46

PDB code     z-score        Ligands              Protein name

1 3wmg(A)     139.8        DMU, TRS.        Crystal structure of an
                                           inward-facing eukaryotic
                                           ABC multidrug transporter
                                           g277v/a278v/a279v mutant
                                           in complex with a cyclic
                                            peptide inhibitor, aCAP

2 3wmf(A)     139.8          DMU.           Crystal structure of an
                                           inward-facing eukaryotic
                                           ABC multidrug transporter
                                           g277v/a278v/a279v mutant

3 IEMDT(A)    139.8          DMU.           Crystal structure of an
                                           inward-facing eukaryotic
                                           ABC multidrug transporter

4 4rhs(A)     126.9    ACT, SIA-SIA-GAL.   Crystal structure of GD2
                                                  bound pltb

5 SPLTB(A)    126.9          ACT.          Crystal structure of pltb

6 STT(A)      126.9          GOL.            Structure of typhoid

7 5luq(A)     111.6                          Crystal structure of
                                              human DNA-dependent
                                           protein kinase catalytic
                                              subunit (DNA-PKcs)
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Title Annotation:Research Article
Author:Lawal, B.; Shittu, O.K.; Abubakar, A.; Kabiru, A.Y.
Publication:Journal of Environmental and Public Health
Date:Jan 1, 2018
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