The prevalence of glucose-6-phosphate dehydrogenase deficiency in Gambian school children

Enzyme activity was measured using a commercial quantitative ELISA kit (Atlas Medical®). It is based on the spectrophotometric measurement of reduced nicotinamide adenine dinucleotide phosphate (NADPH) released during G6PD enzyme activity and, colorimetrically by reduction of tetrazolium salt (550 nm). The readings from the 340 nm measurement were used in the calculations. A 6 mm diameter disc was punched from each dried blood spot (DBS) into a U bottom microtitre plate and eluted with 75 μL of elution agent. NADPH was measured as absorbance at 340 nm[22] in kinetic mode for 15 minutes. Enzyme activity was normalized against the protein content of blood spot eluents determined by measuring absorbance of haemoglobin at 405 nm and expressed as the normalized increase in OD per minute (slope) using the following equation: (∆OD_340nm/∆time)/OD_405nm.

DNA was extracted using protocols for the QiaExtractogen liquid handling robot (QiaGen). Allele polymorphisms were detected by real-time PCR with TaqMan® SNP genotyping assays using ABI PRISM SDS 7500 (Applied Biosystems, Foster City, CA). Oligonucleotide primers and probe genotyping assay mixes for nucleotides A376G, G202A, A542T and T968C, were also obtained from Applied Biosystems. Genotyping assay were performed in a final reaction of 25 μL, containing 12.5 μL of 2× TaqMan Universal Master Mix, 0.5 μL of 40× TaqMan SNP genotyping assay mix and at least 10ηg of genomic DNA in 11 μL of distilled water. The amplification conditions were 2 minutes at 50°C for AmpErase uracil-N-glycosylase activity and 10 minutes at 95°C for Amplitaq Gold activation, followed by 40 cycles of 15 seconds at 95°C for denaturation and 1 min at 60°C for annealing and extension. The samples were run together with the non-template control. Allelic discrimination was performed on fluorescence data using the ABI Prism 7500 allelic discrimination software and the free TaqMan-Genotyper Software (Applied Biosystems, Foster City, CA). Each sample result was verified by examining the PCR curve generated to eliminate false-positive results due to aberrant light emission.

Children were classified on the basis of allelic discrimination patterns as normal, mutant (hemi- or homozygous) or heterozygous (females only) while genotypes were defined for each of the polymorphic A variants; 376, 202, 968, and for the 542 variant. The distribution of G6PD enzyme activity in the sample was analysed using a two-component finite mixture model. Using the population with the higher mean activity as reference, the cut-off for activity in the sample was defined as < −2SD below the mean of this subpopulation. The association between G6PD activity and allele mutation in males and females was examined using Pearson χ². A logistic regression model was used to determine the relationship between allele mutation and a deficient phenotype and the association between haemoglobin, gender and parasitaemia on deficient phenotype. Data was analysed using Stata 12 (College Station Tx).