Background
Malaria is still considered a major public-health problem in the eastern districts of Bangladesh, bordering India and Myanmar. These districts experience a perennial transmission of malaria with two peaks in pre-monsoon (March-May) and post-monsoon (September-November) periods [
1]. In the changing climatic situation and in absence of major malaria vectors, such as
Anopheles minimus and
Anopheles baimaii a number of
Anopheles species have been incriminated and playing a role in the transmission of malaria in the country [
2].
Plasmodium falciparum and
Plasmodium vivax are two main malaria parasites in the country as reported by a nationwide prevalence survey in 2007. The survey showed that contribution of
P. falciparum was 90.18%, followed by
P. vivax (5.29%), and the remaining (4.53%) was mixed infection of these two species [
3].
The Giemsa-stained blood slide using thin and thick smears for malaria parasites has been the gold standard method for nearly a century [
4]. No alternative method still could be established to replace this universally-accepted gold standard method. Such a laboratory technique to confirm the clinical suspicion of malaria is labour-intensive [
5] and sometimes unreliable due to lack of skilled microscopists, limited supplies, inadequate maintenance of microscopes and reagents, and inadequate or absence of quality-control systems [
6].
In recent time, lateral flow immunochromatographic-based rapid diagnostic test (RDT) has been developed for the diagnosis of suspected malaria patients and are widely used in remote areas across the world [
7]. Most RDTs are intended to react with antigens commonly released from or enzymes present in parasitized red blood cells. In the case of
P. falciparum, the water soluble histidine-rich protein-2 (HRP-2) antigen is commonly used as it is specific to
P. falciparum associated infection. Non-falciparum malaria or mixed infections with
P. falciparum are commonly detected by
Plasmodium lactate dehydrogenase (pLDH) [
8,
9]. In the Global Fund sponsored malaria control programme RDT is recommended and being widely used for detecting malaria cases in the endemic areas of Bangladesh [
1].
The molecular detection method, such as polymerase chain reaction (PCR) has been developed to diagnose
Plasmodium spp. and has been performed in several places for routine diagnosis or for evaluating the performance of microscopy or RDT [
10‐
14]. In recent time, real-time PCR method has been established for the quantitative detection of malaria parasites [
15‐
19]. Real-time PCR is reliable and yield high sensitivity and specificity when compared with microcopy or nested PCR [
15,
19,
20].
This study demonstrated a SYBR Green-based modified real-time method to use it as a gold standard, along with conventional microscopy to evaluate four RDTs for diagnosis of malaria from suspected febrile patients. Such a study has never been done before in Bangladesh. The study would provide additional support to the NMCP for monitoring and evaluation of the performances of the diagnostic methods used in their ongoing malaria control programme.
Methods
Study area and population
The study was conducted at Matiranga Upazila (sub-district) of Khagrachari district situated at the south-eastern part of Bangladesh. Febrile patients referred to microscopy for malaria diagnosis at Matiranga Upazila Health Complex (UHC) from May 2009 to August 2010 were enrolled. The recent malaria prevalence survey, Matiranga showed high prevalence of asymptomatic malaria cases (21.6%) [
21].
Sample collection
Five ml of blood was taken from an adult subject and in case of children or minor subjects three ml of blood was obtained through venipuncture by an experienced medical technologist. Two drops of sample were used for preparing thick and thin smear slides, one drop was used for Paracheck RDT, and the remaining samples were preserved in an EDTA tube and stored at -20°C.
Microscopy
The blood film was stained with Giemsa in phosphate buffer saline and examined under the compound microscope at a magnification of ×1,000 for malaria parasites. Blood films were defined as negative if no parasite was observed in 100× oil immersion fields (magnification, ×1,000) on thin film by an experienced microscopist [
22]. Declaring a slide positive or negative and initial speciation was routinely based on the examination of 200 fields in the Giemsa-stained thick film. A slide was considered positive when at least one parasite was found. After finding the first parasite, another 200 fields were completed for any mixed infection. If no parasite was found in 200 oil fields, the slide was considered negative. Density of the parasite was measured from thick blood smears by counting the number of parasites per 200 leukocytes and expressed as parasites/μl. In the case of 10 or less parasites, 500 leukocytes were counted. Each slide was assessed by two independent microscopists; one of them was employed by the study and the other person was posted at Matiranga UHC. A slide was considered positive only when these two microscopists were in agreement. There was a provision for third microscopist posted at the Khagrachari Civil Surgeon's office situated 20 km away from Matiranga UHC for any disagreement between them.
Rapid diagnostic tests
In the present investigation four RDTs (device) were used. These were Paracheck (Orchid Biomedical System, India), FalciVax Pf (Zephyr Biomedicals, India), Onsite Pf (CTK Biotech Inc, USA) and Onsite Pf/Pv (CTK Biotech Inc, USA). Paracheck and Onsite Pf used P. falciparum-specific HRP-2 antigen. FalciVax and Onsite Pf/Pv used P. vivax- specific pLDH together with P. falciparum-specific HRP-2.
All the RDTs were used following the instructions of the manufacturers. 'Paracheck' is being used by the National Malaria Control Programme (NMCP) in the endemic areas and was available at the MUHC. Paracheck test was performed at Matiranga UHC concurrently with the microscopy. The remaining three RDTs were performed using the stored samples as per the instructions of the manufacturers.
DNA was extracted from 200 μl EDTA preserved blood samples using the QiaAmp blood mini kit (QIAGEN, Inc., Germany) following the manufacturer's instructions at the Parasitology Laboratory of ICDDR,B. DNA sample was stored at 4°C until PCR could be completed.
Real-time PCR
Real-time PCR was done by the primer sets described by Perandin
et al[
15] with some modification to a single-plex reaction. Instead of TaqMan probe, SYBR Green I dye was used for visualizing the amplification. PCR condition was also modified slightly to fit with Platinum
® SYBR
® Green qPCR SuperMix-UDG (Invitrogen Corporation, USA) following the instructions of the manufacturer. Purified DNA templates were amplified in a BioRad CFX-96 real time system (BioRad, USA) with a species-specific primer set. Briefly, a 25-μl PCR mixture was prepared using 1 μl of template DNA, 12.5 μl Platinum SYBR Green qPCR supermix (PlatinumR
Taq DNA polymerase, SYBR Green I dye, Tris-HCl, KCl, 6 mM MgCl2, 400 μM dGTP, 400 μM dATP, 400 μM dCTP, 800 μM dUTP, uracil DNA glycosylase, and stabilizers), 320 nM concentration of each of parasite species-specific primer set. Amplification and detection were performed as follows: 50°C for 2 min and 95°C for 2 min. After that 95°C for 1 min, 58°C for 1 min and 72°C for 1 min 30 sec for a single cycle were performed. 40 cycles were considered for
P. falciparum and 35 cycles for
P. vivax. The plate read was taken after the extension at 72°C. The melt curve was prepared from 50°C to 95°C with an increment of 0.5°C each after five seconds.
To establish the minimum number of parasites detectable by the Plasmodium SYBR Green assay (detection limit), blood samples from two patients infected, respectively, with P. falciparum (one patient) and P. vivax (one patient) were collected, and parasitaemia was calculated using 200 WBC count as reference. The infected blood samples were diluted with uninfected erythrocytes from healthy individuals with known baseline erythrocyte counts. Ten-fold serial dilution was made to obtain a final parasitaemia of 1% (1 parasite/μl of blood) for each sample. All DNA aliquots purified from the dilutions were treated in duplicate for real-time PCR assay. To estimate the analytical specificity of the Plasmodium real-time PCR assay, DNA from in vitro culture samples of other protozoan parasites, such as Entamoeba histolytica and Leishmania donovani were used. The clinical sensitivity and specificity of the modified Plasmodium real-time PCR assay for detecting and identifying malaria parasites were calculated on 338 whole-blood samples, microscopy as the gold standard and vice- versa.
Analysis of data
The performance of each method was calculated by means of sensitivity, specificity, positive predictive value (PPV), and negative predictive value (NPV) using microscopy and modified real-time PCR as gold standard. SPSS software version 11.5 (SPSS Inc., USA) was used for calculating the kappa coefficient (k) of the tests for each association using the X
2 test. Sensitivity, specificity, positive predictive value and negative predictive value were calculated using the 'diagt' command of the STATA software version 10 (Stata Corp, USA)[
23].
Ethical approval
The study was approved by the Research Review Committee and Ethical Review Committee of ICDDR,B. Approval was also obtained from the NMCP for the study. Informed consent was obtained from all adult subjects, and assent was obtained from the legal guardians in the case of minor subjects before the collection of blood sample. Good clinical and laboratory practices were followed in all the procedures.
Discussion
Although in Bangladesh,
P. falciparum and
P. vivax are the two common prevalent parasites, the majority of malaria cases are caused by
P. falciparum[
1]. However, their ratio varies from time to time. During the nationwide malaria prevalence survey in 2007 based on Falcivax RDT, 90%
P. falciparum infection was found and the remaining 10% infection was due to pure
P. vivax or mixed infection of these two parasites although the performance of that RDT (Falcivax) was not evaluated against any gold standard method [
3].
This study demonstrated the establishment of pre existing real-time PCR assay modified with SYBR Green dye for the detection of
P. falciparum and
P. vivax as an alternative gold standard method for evaluating RDTs used for the diagnosis of malaria. Simultaneously, the performance of microscopy can also be evaluated by this SYBR Green-based PCR method. The original TaqMan-based real-time PCR method was 100% sensitive and specific using nested PCR as gold standard [
15]. But in the present study more than 95% of sensitivity and specificity was obtained for both
P. falciparum and
P. vivax using microscopy as a gold standard. The modified real-time PCR method detected eight
P. falciparum and
P. vivax mixed infections, of which two were detected by microscopy, Falcivax and Onsite Pf/Pv RDT. On the other hand microscopy detected three mixed infections of which modified real-time PCR could detect two and one by Falcivax and Onsite Pf/Pv tests respectively. One sample detected as
P. vivax by microscopy was detected as mixed infection by modified real-time PCR, Falcivax and Onsite Pf/Pv tests. At the same time one sample was found to be
P. vivax in all other tests, but detected as
P. falciparum by microscopy. Two samples were detected negative by microscopy and all the RDTs, but found to have
P. falciparum in real-time PCR. These two samples were missed in microscopy and RDTs perhaps due to the low number of parasite counts [
15,
24].
This study was conducted among the symptomatic febrile patients in a high-endemic area. RDTs can play a key role in rapid diagnosis and, hence, prompt treatment of malaria. As RDT can be conducted immediately in the field clinic or even in the field level by the health workers while the patient is present, the most important point for the villagers is the knowledge that they are infected with malaria parasite. On the contrary, the delay in the results of microscopic diagnosis is a serious obstacle for the operation of a malaria control programme in remote areas. Although RDTs have some limitations, all the four tests evaluated had high sensitivity and specificity. The high NPV allow us to confidently diagnose negative test patients as non-malaria patients [
25]. Thus, the risk of missing an infected individual is less by the RDTs used in this evaluation. In a similar study in India, high NPV was also recorded for Falcivax RDT [
13].
Overall, 55.9% of the febrile patients with suspected malaria in the present study had a positive blood slide, indicating that over half of the suspected cases referred to this hospital (Matiranga UHC) had malaria. A high percentage of malaria cases among the febrile cases of this area could be due to a high prevalence of asymptomatic malaria cases at the community [
21].
Pf-HRP 2 based Paracheck is currently being used in the country's NMCP, although there is a necessity of a RDT for detecting multiple malaria infections in the country [
1]. In the present study Parachek showed high sensitivity and specificity compared to a study in Malawi where low specificity was reported [
26]. However, since the control programme is now targeting for RDTs that can detect multiple infections, this study could provide a valuable guideline to them.
Onsite duo as newly developed test had never been evaluated earlier in any part of the world gave satisfactory results in the present study. Although Onsite Pf/Pv failed to diagnose some P. falciparum positive sample which undoubtedly affects its sensitivity compared to its counterpart Falcivax. However, Onsite Pf/Pv gave almost a similar result as like as Falcivax for detecting P. vivax.
Low sensitivity of the two RDTs (Falcivax and Onsite Pf/Pv) for the detection of
P. vivax compared to real-time PCR assay in this present study is similar to studies published earlier [
20,
26]. This could be due to the inherent limitations of pLDH assay to detect low parasitaemia in the clinical specimens [
27]. Miscroscopists similar to RDTs also missed
P. vivax cases compared to real-time PCR assay perhaps due to the same reason (low parasitaemia)[
28].
RDTs do not depend on the operator like microscopy. It was evolved to overcome or reduce the limitations of microscopy. They have brought a revolution in the field of malaria diagnosis. However, these must achieve > 95% sensitivity to prove their usefulness [
29]. It has been estimated that over 70 million RDTs are sold across the world. There are a number of companies producing RDTs for the diagnosis of malaria which was initiated by a single company in 1993 [
30]. The world health organization listed approximately 50 RDTs, of which only a few had PvLDH antigen-based tests that distinguish between
P. falciparum and
P. vivax are commercially available [
26].
Acknowledgements
This research study was funded by ICDDR,B and its donors which provide unrestricted support to ICDDR,B for its operations and research. Current donors providing unrestricted support include: Australian Agency for International Development (AusAID), Government of the People's Republic of Bangladesh; Canadian International Development Agency (CIDA), Swedish International Development Cooperation Agency (Sida), and the Department for International Development, UK (DFID). We gratefully acknowledge these donors for their support and commitment to ICDDR,B's research efforts.
The authors are grateful to NMCP for their permission to conduct the study in their facilities and also for providing Paracheck RDT. The authors are also grateful to CTK Biotech Inc, USA, for providing 'Onsite Pf' and 'Onsite Pf/Pv' RDT as a donation. The authors are also indebted to the people of Matiranga who had consented to participate in the study and the doctors and staff of Matiranga UHC for their extended supports. The authors also appreciate the contribution of Mamun Kabir, Khaja Mohiuddin, A. E. M. Rubayet Elahi, Milka Patracia Podder, Shihab U. Sobuz, and Md. Gulam Musawwir Khan for their valuable contributions to the study.
Competing interests
The authors declare that they have no competing interests.
Authors' contributions
MSA conceptualized and designed the study, collected and identified samples, analysed data, drafted the manuscript and made final revisions. MSA, ANM, WAK, NI, MJK, HK, DS, RH did sample analysis and made critical revision of the manuscript. SM organized the field activities, analysed data and helped revise the manuscript. MSA and RH drafted the manuscript. All the authors read the final version of the manuscript and approved.