Heterogeneous malaria transmission in long-term Afghan refugee populations: a cross-sectional study in five refugee camps in northern Pakistan

Study participants were selected from five Afghan refugee camps in Mardan (Baghecha, Kaghan and Jalala camps) and Peshawar (Adezai) districts in the province of Khyber Pakhunkwa (KPK) in Pakistan, as well as the Zangal Patai camp in the Malakand agency tribal area (Fig. 1). Camps were established in the late 1980s with some refugees being resident for more than 30 years at the time of the survey. The surveys took place between 24 June and 19 September, 2010 to coincide with the main P. vivax transmission season and before the P. falciparum transmission season, which typically peaks in late October [5, 9, 16]. The main vectors in the area are Anopheles stephensi and Anopheles culicifacies and the majority of the malaria infections are due to P. vivax [4]. The area is characterized by sandy and marshy land and is well irrigated for sugar cane, wheat and rice production. Houses are primarily constructed with rocks, bricks and mud and animal ownership is common. Free primary health care is provided at basic health units (BHUs) established in each camp and run by the UN High Commissioner for Refugees. Malaria testing and treatment of microscopically confirmed cases is provided free according to national guidelines [15].

Sample size calculations for the survey were derived based on estimating anti-malarial antibody seroconversion rates (λ) of 0.01 with a residual standard deviation less than 0.25, which resulted in a sample of three people per household with a minimum of 167 households [17, 18]. A numbered list of all current households was obtained for each camp and the total number of people per age group in each household was recorded to provide a sampling weight for the data. Two-hundred households per camp were randomly selected to allow for refusal and absenteeism. One person from each of three age groups (one to five, six to 20 and >21 years) per household was randomly selected for collection of blood samples.

The household heads in all selected households were approached for written informed consent and questionnaires were administered to collect information on household characteristics, including wealth indices, travel history, malaria control behaviour, and demographic information. Finger-prick blood samples were collected on Whatman 3 mm filter paper (Maidstone, UK) from the selected individuals for subsequent laboratory analysis after written consent was obtained. The CareStart Pf/Pv combo (Access Bio, Inc. NJ, USA) RDT was performed to detect current malaria infections with P. vivax (pLDH) and/or P. falciparum (HRP2). All individuals found to be RDT positive were referred to a BHU for full evaluation and for appropriate treatment. Blood was also collected onto Whatman 3 mm filter paper (Maidstone, UK) for laboratory analysis.

Filter-paper blood spots were dried in the field and stored with desiccant at −20 °C and shipped to London for analysis. Antibodies to P. falciparum and P. vivax Apical Membrane Antigen-1 (AMA-1) and Merozoite Surface Protein-1₁₉ (MSP-1) were detected using enzyme-linked immunosorbent assay (ELISA) as previously described [11]. In each camp, individuals positive by RDT and a random selection of 120 RDT-negative individuals were assayed by a nested, species-specific PCR as previously described [19]. Due to the higher malaria prevalence observed in Jalala camp, all samples were analysed by PCR. Briefly, DNA was extracted using chelex-saponin and genus-specific primers were used in the nest-1 reaction and two separate nest-2 reactions were conducted using primers specific for P. vivax and P. falciparum.

Data analysis was conducted using Stata v12.0 (Stata Corp LP, TX, USA) and R v3.2 (R-Project, USA) statistical software. Duplicate ELISA OD values were averaged and normalized against the positive control sample on each plate. OD data were then converted to antibody titres, expressed in arbitrary units (AU/ml), using a standard curve obtained from hyperendemic control sera. Seropositivity was defined by fitting a mixture model to normalized OD values [20]. The model assumed two Gaussian distributions, one for seronegative values and the other seropositive values. The mean OD plus three standard deviations of the seronegative values for each species and antigen was used as the cut-off value for seropositivity. An individual was considered to be seropositive if they responded to at least one of the two antigens tested for each species [21]. Seroprevalence was stratified into age groups and the seroconversion rate (SCR) was estimated by fitting a reverse catalytic conversion model under a binomial sampling assumption [17]. PCR prevalence was calculated using a bootstrap approach to avoid bias associated with the sampling approach. Briefly, a subset of samples assayed by PCR was randomly selected with replacement according to RDT positivity. PCR prevalence of the sample was determined and repeated 10,000 times. The mean of the bootstrapped estimates provided the overall PCR prevalence per camp and 95 % confidence intervals were calculated according to the Chen-Shao method [22].

Principal component analysis was used to generate a score for socio-economic status (SES) based on household asset ownership data and grouped according to quintiles [23]. Logistic regression was used to assess risk factors for both P. falciparum and P. vivax using the survey command, weighted for household population size, and adjusting for clustering within camps. Spearman’s rank correlation coefficient was calculated to compare diagnostic tools within camps. Hotspots were determined assuming a Bernoulli model with SatScan software v9.2 (Harvard, Boston, USA). Elliptical and circular windows were used allowing for a maximum spatial cluster size of both 50 and 25 % of the population at risk. Those households showing evidence of a significantly (p < 0.05) increased prevalence compared to the rest of the camp by any of the scans were considered to be part of a hotspot [11, 24]. Separate scans were conducted for sero- and RDT positivity for both P. vivax and P. falciparum and results were analysed using ArcGis v10.2 (ESRI, CA, USA). Due to the sub-set of samples analysed, spatial analysis was not conducted on PCR results.

Ethics approval for the study was granted by both Peshawar University (#02/EC/Pharm) and the London School of Hygiene and Tropical Medicine (#5715). Individual written informed consent was sought from heads of included households, and from all selected participants by signature. Consent for children under the age of 18 was provided by a parent/guardian.