Comparative evaluation of two rapid field tests for malaria diagnosis: Partec Rapid Malaria Test® and Binax Now® Malaria Rapid Diagnostic Test

Background About 90% of all malaria deaths in sub-Saharan Africa occur in children under five years. Fast and reliable diagnosis of malaria requires confirmation of the presence of malaria parasites in the blood of patients with fever or history suggestive of malaria; hence a prompt and accurate diagnosis of malaria is the key to effective disease management. Confirmation of malaria infection requires the availability of a rapid, sensitive, and specific testing at an affordable cost. We compared two recent methods (the novel Partec Rapid Malaria Test® (PT) and the Binax Now® Malaria Rapid Diagnostic Test (BN RDT) with the conventional Giemsa stain microscopy (GM) for the diagnosis of malaria among children in a clinical laboratory of a hospital in a rural endemic area of Ghana. Methods Blood samples were collected from 263 children admitted with fever or a history of fever to the pediatric clinic of the Agogo Presbyterian Hospital. The three different test methods PT, BN RDT and GM were performed independently by well trained and competent laboratory staff to assess the presence of malaria parasites. Results were analyzed and compared using GM as the reference standard. Results In 107 (40.7%) of 263 study participants, Plasmodium sp. was detected by GM. PT and BN RDT showed positive results in 111 (42.2%) and 114 (43.4%), respectively. Compared to GM reference standard, the sensitivities of the PT and BN RDT were 100% (95% CI: 96.6-100) and 97.2% (95% CI: 92.0-99.4), respectively, specificities were 97.4% (95% CI: 93.6-99.3) and 93.6% (95% CI: 88.5-96.9), respectively. There was a strong agreement (kappa) between the applied test methods (GM vs PT: 0.97; p < 0.001 and GM vs BN RDT: 0.90; p < 0.001). The average turnaround time per tests was 17 minutes. Conclusion In this study two rapid malaria tests, PT and BN RDT, demonstrated a good quality of their performance compared to conventional GM. Both methods require little training, have short turnaround times, are applicable as well as affordable and can therefore be considered as alternative diagnostic tools in malaria endemic areas. The species of Plasmodium cannot be identified.


Background
Half of the world's population is at risk of malaria, with an estimated 243 million cases worldwide out of which 85.6% cases occur in Africa [1]. The World Health Organization (WHO) estimated that 767 000 deaths occurred in Africa in 2008 of which almost 90% were children under five years [1]. Prompt parasitological confirmation by microscopy or alternatively by rapid diagnostic tests (RDTs) is recommended for all patients with suspected malaria before treatment is started [1]. This is to prevent the misuse of antimalarial drugs especially Artemisinin-based combination therapies thereby preventing the possible development of resistance in the parasite to these drugs. Treatment solely on the basis of clinical suspicion should be considered only when parasitological diagnosis is not accessible [1]. Thus, it is of concern that poor diagnostic standards such as the lack of skilled microscopists and inadequate or absence of quality control systems [2] continue to hinder effective malaria control.
Another major contributing factor is that the laboratory diagnosis of malaria has up to now relied nearly exclusively on light microscopy which is a valuable technique when performed correctly but unreliable and wasteful when poorly executed. A better utilization of microscopy and the development of alternative diagnostic techniques could substantially improve malaria control [3]. This study aimed at evaluating and comparing the novel Partec Rapid Malaria Test ® (PT) (Partec GmbH, Münster, Germany) and the recently established Binax Now ® Malaria Rapid Diagnostic Test (BN RDT) (Binax, Inc., Portland, ME, USA) in malaria diagnosis among children from an endemic area using Giemsa stain microscopy as the reference standard. In a first report we compared PT with GM in a separate collective of patients using a real time PCR assay as reference standard [4]. In this study we focused on the assessment of test result quality and applicability under the field conditions of a rural hospital laboratory.

Study site
The study was conducted at the Agogo Presbyterian Hospital. It is located in the rural Asante Akim North District of the Ashanti Region of Ghana, West Africa and is the principal hospital of the district. The district is located in the eastern part of Ashanti Region and covers a land area of 1,160 km 2 with an estimated population of about 142,000 (projection from 2000 Population Census). Over 40% of the population is under 15 years and over 50% are under 20 years of age. The microscopically confirmed incidence of malaria in children under five who reported at the under-five clinic of the Agogo hospital was 265 per thousand in 2008 (unpublished data, Biostatistics Dept, Agogo Presbyterian Hospital).

Study population
Between June and December 2008 (i.e. from the beginning of the rainy season to the early dry season), 263 cases were enrolled into the study. Samples were obtained from children attending the pediatric clinic of the hospital for the first time with fever or a history suggestive of malaria but without previous antimalarial treatment within two weeks of attending the hospital. Patients diagnosed with malaria were treated with Artesunate -Amodiaquine or Artemether -Lumefantrine as second line treatment representing the Ministry of Health/National Malaria Control Programme approved Artemisinin-based combination therapy for the treatment of uncomplicated malaria in Ghana.

Ethical Approval
Ethical approval for the study was obtained from the Committee on Human Research, Publication and Ethics (CHRPE) of the School of Medical Sciences, KNUST-Kumasi. After information and appropriate explanations parents or legal guardians of all participants willing to participate in the study had to give their consent by appending their signature or thumbprint to the informed consent form before any study related procedures were done. Internationally accepted Good Clinical and Good Laboratory practices were applied in all procedures.

Sampling
A maximum of 0.5 ml capillary blood was taken from each child into an EDTA tube labelled with the patient's barcode and pathology number. These samples were examined immediately using the three methods (GM, BN RDT and PT). All three tests were done immediately and examined by well-trained and competent laboratory staff. For GM, the test was examined independently by two expert microscopists in two different rooms with each not knowing the result of the other. In the case where the two microscopic results were discordant, a third expert reader was employed by an independent slide coordinator. The result of the third reader was then considered as the final result. Written results were communicated immediately to the clinicians.

Giemsa-stained blood film
Thick and thin blood films were prepared using standardized blood volumes of 10 μl and 2 μl, respectively. They were air-dried (thin film was fixed in absolute methanol), heat fixed and both stained with 10% Giemsa working solution for 12 minutes. A malaria blood film was considered negative after 100 high power fields (HPF) has been examined and no parasite observed. If parasites were observed, asexual malaria parasites were counted against 200 white blood cells (WBCs) on the thick film but all parasites in a final HPF were counted even if a count of 200 WBCs had been exceeded. The parasite count per microliter of blood was obtained by using the formula: (Parasite count/200WBC) × Absolute WBC count [5]. If parasite density was more than 100 parasites/field in a thick film, the thin film was used for the count. Upon the observation of asexual malaria parasites, parasitized red blood cells (RBCs) were counted against 1,000 RBCs. The parasite count per microliter of blood was obtained by using the formula: (Parasite count/1000RBC) × Absolute RBC count [6]. The thin film was used for species identification of detected malaria parasites. Absolute WBC and RBC counts were estimated by using the Sysmex KX 21N hematology auto analyzer (Sysmex Corporation, Kobe, Japan). In addition, gametocytes, schizonts and other blood parasites, when present, were reported to the clinicians. Known positive and negative samples were used as controls for freshly prepared Giemsa working solution each day.

Partec Rapid Malaria Test ®
The Partec CyScope ® (Partec GmbH, Münster, Germany) is a microscope that has two light sources: in addition to the option of normal light microscopy, a fluorescence light detection through incident UV light can be applied. It uses readily-prepared and ready to-use test slides labelled with an unspecific DNA-binding fluorescent dye (4'-6-Diamidino-2-phenylindole (DAPI); emission 443 nm) that detects intraerythrocytic Plasmodium DNA [4] resulting in a bright intracellular dotshaped fluorescence if the RBCs are infected with malaria parasites. The test was performed following manufacturer's instructions [7]. 5 μl of well mixed capillary blood was placed on the dye labeled area of a slide with the patients' pathology number, cover slipped, incubated at room temperature for a minute and observed under the 100× objective (oil immersion) under LED UV light (365 nm). The presence of bright shiny intracellular tiny dots observed under the UV light indicated the presence of malaria parasites in erythrocytes. To prevent the slides from drying out, they were kept in a wet chamber. Parasites counts were done as described in the GM method above. If parasite density was more than 100 parasites/field in a thick film, an approximate count was done by counting a quarter of the field and multiplying by four to get an approximate parasite count per field. This figure was used to calculate the parasite density per microliter. Positive and negative controls were done for each batch of test kits.

Binax Now ® Rapid Diagnostic Test
The BN RDT (Binax, Inc., Portland, ME, USA) is an immunochromatographic membrane assay that uses monoclonal antibodies to detect P. falciparum specific histidine rich protein 2 (HRP-2) and a panmalarial aldolase common to all four human pathogenic species in venous and capillary blood specimens [8]. This test was done as described by Wongsrichanalai et al. [9]. 15 μl of blood was placed on the purple sample pad; two drops of test reagent were added to the lower absorbent white pad located immediately below the sample pad and four drops to the absorbent white pad up. Lysed blood wicked up to the base of the upper white absorbent pad in a few minutes, when the booklet was closed. The results were read through the viewing window of the device 15 minutes after closing the window. The presence or absences of test lines were used to determine positive and negative results [10] (Table 1). Positive and negative controls were done for each batch of test kits.

Statistical analysis
Data were double-entered into a predesigned electronic database using Epi info version 6.04 dfr (Center for Disease Control, Atlanta, GA, USA) and cleaned regularly. Data was exported to Stata/SE9.0 statistical software (Stata Corporation, Texas USA) for analysis. Sensitivities, specificities, positive predictive and negative predictive values were determined for the various tests and compared with one another. A p-value less than 0.05

Patient recruitment
From June to December 2008 a total of 263 children (147 males and 116 females) up to 16 years, admitted with fever or a history suggestive of malaria were included in the study with a mean ± SD age of 7.3 years ±3.4 years (range: 3-16 years).

Giemsa stain microscopy
Overall, GM expert microscopy (  (Table 3). Table 3 shows the degree of agreement (kappa), with a 95% confidence interval, observed between the different test methods. Overall, there was a high degree of agreement between the test methods and the reference standard.

Discussion
In this study we assessed the field performance of the PT and BN RDT in a rural Ghanaian hospital laboratory using conventional Giemsa stain thick and thin blood films of pediatric specimens as reference standard. Only few studies in other endemic areas have been conducted specifically in children so far [12][13][14][15][16]. In one study an increased sensitivity of a HRP-2 assay in children compared to adults was demonstrated. This was attributed to lower immunity and possibly less interference by antibodies [17]. Despite this, there is concern that the benefits of parasitological confirmation in children under 5 years may be outweighed by the risks of not treating children with false negative tests [18]. Studies conducted earlier on BN RDT showed a low sensitivity (61.5%) for the detection of pure P. malariae and P. ovale infections [8]. We found false negative results of BN RDT for only two non-P. falciparum infections with low parasite counts (Pm: 24 parasites/μl and Po: 16 parasites/μl) and thus this might be inadequate to confirm or refute this point. The BN RDT however, has been shown to have a very good sensitivity (100%) for the detection of pure P. falciparum infection [9]. P. falciparum accounts for almost 99% of malaria infections in the study area (unpublished data, Biostatistics Dept, Agogo Presbyterian Hospital) and, therefore, the low sensitivity of the BN RDT for non-P. falciparum malaria may not be a serious cause for concern in this area and most parts of sub-Saharan Africa where malaria infection is predominantly caused by P. falciparum [19]. A slight cause for concern might be the number of steps (about 6 steps) involved in performing the test as compared to the four-step test of other RDT formats [20]. However, with adequate training this concern can be addressed. The BN RDT detects the presence of plasmodial antigens HRP-2 and pan-Plasmodium aldolase [21]. The detection of 10 falsepositive results could be attributed to one main observation made in earlier studies. It is well documented that the HRP-2 antigen can persist up to 28 days after treatment [22,23]. Even though only untreated patients were enrolled in this study, reliability of information obtained from mothers/guardians on this might be questionable. This assumption could have contributed to the increased numbers of false positive tests. In addition this assay appears to be an unsuitable tool for monitoring treatment of malaria as previously discussed by Murray et al [24]. The BN RDT has also been shown to detect parasite levels > 20 parasites/μl for P. falciparum and ≤ 100 parasites/μl for P. vivax [8]. False negative results could be attributed to the fact that parasite antigen levels were too low to be detected as a result of very low parasitaemia or by semi-immune parasite carriers with low parasitaemia.
Overall the test is simple to perform, rapid (< 15 minutes), easy to interpret, requires less training, needs no laboratory setup and thus it is applicable for field conditions [8,9,21]. The test has also been shown to be heat stable and performs very well at temperatures up to 45°C [25]. On the other hand, it has a poor detection rate for non-P. falciparum infections and has a higher false positive rate due to the persistence of the antigen target HRP 2 [8,9,26].
PT uses a fluorescent dye 4'-6-Diamidino-2-phenylindole (DAPI) which detects intracellular double stranded DNA which is present within Plasmodium-infected erythrocytes. The bright shiny dots within infected erythrocytes under UV light is extremely characteristic for malaria and has a very high PPV in areas mainly endemic with P. falciparum [4]. One major limitation of PT is the disability of specific identification of Plasmodia and the differentiation of the species. Compared to GM, PT exhibited four false-positive results which have not been further investigated. PT could also be more sensitive than GM in detecting low number of parasites [4]. The presence of artifacts such as non-specific aggregated DAPI, immature erythrocytes or bacterial cells might have been misinterpreted as plasmodial DNA. The performance characteristics of the tests were very similar as indicated in their sensitivities, specificities, PPV and NPV with very good agreements to the GM reference standard (Table 3). Our study findings correlate well with the results of a study conducted in Sudan for adults using the Partec CyScope ® when compared only with conventional Giemsa stained microscopy [27] as well as with our first report comparing this malaria test in another patient's collective [4]. In this first study we could attest to the fact that the PT has a high sensitivity and specificity by referring to the highly sensitive gold standard RT-PCR which, however, cannot be applied in field studies in contrast to the PT assay [4]. Both studies [4,27] confirmed that PT requires very little training and has a short turnaround time of averagely 5 minutes per test. In addition our findings regarding PT performance characteristics and applicability under field conditions were confirmed by a study conducted in Uganda [28]. This study also underlines the disability of specific identification and differentiation of Plasmodia species as the disadvantage of PT. However, the characteristic fluorescence of infected erythrocytes has a very high PPV in areas mainly endemic with P. falciparum.
Thus we value PT analog to GM thick film as a useful screening method where positive and doubtful results need to be completed by GM thin film examination for confirmation and accurate identification of species later. This strategy takes also into account that Giemsa staining and microscopy is a very elaborate and challenging procedure when performed accurately in a high quality level.
Parasitaemia is used to guide treatment, thus underestimation could have significant ramifications for malaria patients. Parasite counts obtained from PT were significantly lower than those obtained from GM. It is unlikely that parasites are hidden during Giemsa stain microscopy, since adequate preparation of the slide ensures visibility through all planes of focus. The lysis of the red blood cells during the staining process reveals the parasites and ease the detection [29]. The Partec Rapid Malaria Test ® employs fluorescence in which red blood cells are not completely lysed, therefore, they may lie on each other or overlap with each other thereby preventing parasites in red blood cells that may be lying beneath other cells from being identified and counted.
The World Health Organization Sexually Transmitted Diseases Diagnostics Initiative (SDI) has developed the ASSURED criteria as a benchmark to decide if tests address disease control needs: Affordable, Sensitive, Specific, User-friendly, Rapid and robust, Equipment-free and Deliverable to end-users [30]. Even though this criteria was developed as a benchmark for the evaluation of RDTs for sexually transmitted infections such as syphilis, it can also be used as a benchmark for the evaluation of RDTs for other diseases such as malaria (Table 4). In rural endemic areas where majority of the people are poor, these tests are affordable enough to be accessed in the health centers and homes.
The accepted level of sensitivity for a rapid diagnostic test in diagnosing malaria is a sensitivity of 95% [31]. Compared to the reference standard, both methods were sensitive and specific enough to be used as diagnostic tools for the diagnosis of malaria in endemic areas.
Both methods require little training and the BN RDT can withstand temperatures up to 45°C [25], making it quite useful for tropical conditions and does not require any equipment. The PT is battery operated, portable and can thus be carried for field work and to places where there may be no regular electricity.
There is the need therefore to expand malaria diagnostic services as part of a greater framework of health system strengthening within resource-limited settings. Increasingly, countries and implementing partners have identified that limited diagnostic capacity represents a major barrier to implementation and sustainability of prevention, treatment and care programs for malaria [32]. The PT and BN RDT, therefore, present as very good tools in the prevention, treatment and care programs for malaria.

Conclusion
In this study we demonstrated comparable and acceptable performance and operational characteristics of PT, BN RDT and conventional GM with very good agreements with each other. PT and BN RDT require little training only, have very short turnaround times, are applicable under field conditions as well as affordable even in rural areas. Therefore both methods can be considered as alternative diagnostic tools in malaria endemic areas in addition to or instead of GM.

Recommendations
• This study has found the PT to be a reliable diagnostic tool that is sensitive and specific in diagnosing falciparum malaria. Since this is the predominant species causing most mortality and complications in Ghana and sub-Saharan Africa, it is relevant and useful. It is expected that the CyScope ® will show similar results for other malaria species especially P. vivax, but this could not be ascertained by this study. Further studies are needed to determine its effectiveness in diagnosing other Plasmodium species.
• Based on the ASSURED criteria and the need to expand malaria diagnostic services as part of a greater framework of health system strengthening within resource-limited settings [32], the PT and BN RDT can be considered as a point-of-care diagnostic device for resource limited endemic areas.

Limitations
• In Africa over 70% of malaria cases do not present initially to health facilities but diagnosed and managed at home with traditional remedies or drugs bought from local shops [33]. Patients only attend health centers after self-treatment fails [34]. This

Disclaimer
The findings and conclusions in this paper are those of the authors and do not necessarily represent the views of any of their affiliated Research Institutions.