Estimating malaria parasite density: assumed white blood cell count of 10,000/μl of blood is appropriate measure in Central Ghana

The study was carried out on laboratory data from the Kintampo North Municipal and South District of Ghana, which cover in total, an area of 6,883 sq km with a population of approximately 189,958, and also from Wenchi Municipality and Tain District, which cover an area of 7,619 km² with an approximate population of 166,641 (Ghana Districts). The study area is located within the forest-savannah, transitional ecological zone in Ghana. Studies in the area showed 50 % prevalence of malaria parasitaemia among children less than 10 years of age (symptomatic/asymptomatic). Malaria transmission is perennial, with entomological inoculation rate of 269 infective bites per person per year [12]. Plasmodium falciparum malaria predominates in this area with seldom malaria resulting from Plasmodium malariae and Plasmodium ovale. Mean monthly temperatures range between 18 °C and 38 °C and rainfall averages 1,250 mm per annum for the sites selected, making conditions optimal for vector abundance. Plasmodium falciparum resistance to chloroquine was greater than 40.0 %, similar to that recorded in other parts of the country [13]. Malaria microscopy is available for malaria diagnosis in hospitals in the selected site. Malaria rapid diagnostic test (RDT) kits are supposed to be used in peripheral health centres. Anti-malarials, particularly ACT, for uncomplicated malaria are registered to be sold over the counter in the study area and other parts of Ghana.

The data analysis was carried out on laboratory results obtained from all children under five years old, recruited into three major malaria studies carried out in KHRC for the period of April 2009 to March 2011. Children less than five years of age were selected because they are the most vulnerable group and represent the population mostly recruited in the majority of clinical trials of anti-malarials and malarial vaccines in sub-Saharan Africa. The children ranged from day-old babies to those aged five years depending on the design of the various studies.

The studies adopted were approved by the ethical review committees of the Ghana Health Service, London School of Hygiene and Tropical Medicine, KHRC, Noghuchi Memorial Institute of Medical Research and The Food and Drugs Board, Ghana. Community entry involved explaining the studies to key community opinion leaders followed by community durbars/meetings. At these meetings, the study aims, objectives, risks and benefits were explained to all participants and informed consent was sought from all mothers whose children participated in the studies. All data collected were kept in locked cabinets to ensure confidentiality.

Blood samples were collected from children recruited into the three major malaria-based studies in KHRC. The recruitment processes were done with the support of the established Health Demographic Surveillance System (KHRC-HDSS). Capillary blood samples by finger-prick were collected from the participants on their study visit days and on any other days participants had fever or an axillary temperature greater or equal to 37.5 °C, for a period stated and approved by the various study protocols, and were referred for further treatment and management. Samples were collected into 0.5 ml microtainers ethylenediaminetetracetic acid (K2EDTA-BD, USA) and were transported to the clinical laboratory in the research centre in Kintampo for analysis.

Two blood slides were prepared for each sample that came to the laboratory. Each slide had a measured volume of 6 μl of blood for thick film and 2 μl for the thin film. Ten percent (1:9 ml) for 10 min and 3 % (3:97 ml) for 45–60 min fresh, working Giemsa stains were prepared with already prepared stock of Giemsa-staining solution and working Giemsa buffer prepared from buffer tablets. Thin and thick blood smear were stained with Giemsa after fixing the thin smear with absolute methanol. The 10 % Giemsa stain was used to stain one of the two slides for preliminary slide reading to release results for participant management and treatment. The slide stained with 3 % was given out by the slide coordinator to two competent, independent malaria microscopists. A positive smear was included with each new batch of working Giemsa stain for quality control.

The entire smear was first screened at a low magnification (10X × 40X objective lens) to detect suitable fields with even distribution of WBC (10–20 WBC/field) [9, 12]. Smears were then examined using X100 oil immersion. At least 100 high power fields were examined before a thick smear was declared negative. Plasmodium falciparum parasites were counted per 200 or 500 leukocytes, which were used to estimate the parasite density per microlitre of blood. Thin films were examined to confirm the species identification on the thick film. Blood slide was declared positive when a concordant result was produced by two competent microscopists.

The full blood counts (FBC) analysis for each participant’s sample was analysed using the ABX Micros 60 (Horiba ABX, Montpellier, France). Daily internal quality controls and the scheduled external quality assessment programme were adhered to as a quality measure. Two results for all analysed samples were printed. One was filed in the laboratory and the other dispatched into participant’s folder.

= (Number of parasites counted/WBC counted) × WBC count/ μL of participant.

Also, parasite densities for all participants were calculated using assumed WBC of 5.0 × 10(9)/L, 6.0 × 10(9)/L, 8.0 × 10(9)/L and 10.0 × 10(9)/L of blood; all set by WHO to be used conveniently in facilities which lack the tools to determine patients’ absolute FBC values.

The summary of the methods employed for sample collection and laboratory analyses is illustrated in Figure 1.

Data was checked for completeness and consistency and all queries resolved after double data entry. All negative blood slide results were removed from the data set for analysis. Clean data were analysed using the statistical programs STATA (version 11; Stata Corp., TX USA) and GraphPad PRISM version 5.0 (GraphPad Software, Inc). P-values under 0.05 were considered significant and 95 % CI of geometric means that did not overlap was considered a significant difference.

The ages of all participants were not stratified into groups. This did not make it possible to compare differences at the possible age groups less than five years. Information on sexes was not included for analysis.