Comparison of glucose-6 phosphate dehydrogenase status by fluorescent spot test and rapid diagnostic test in Lao PDR and Cambodia

G6PD deficiency was assessed by the FST (Trinity Biotech Plc, IDA Business Park, Bray, Co Wicklow, Ireland), the CareStart G6PD rapid diagnostic test (G6PD RDT) screening kit (Access Bio. Inc., New Jersey, USA), and by quantitative spectrophotometry (Trinity Biotech, Ireland). Spectrophotometry results were adjusted for individual haemoglobin levels (Hb) as measured by HemoCue^® (HemoCue Hb301; HemoCue AB, Ängelholm, Sweden) in the laboratory. All G6PD assays were performed independently and blinded to G6PD status of the participant.

A total of 5 μL of whole blood was added to 100 μL G-6-PDH substrate solution. A first aliquot was immediately spotted onto filter paper and the remaining solution incubated at room temperature. A second and a third drop of blood-substrate mixture were blotted after 5 and 10 min of incubation. The filter papers were air dried for approximately 30 min and subsequently read under UV light. A sample with normal enzyme activity showed moderate to strong fluorescence after 5 min, and strong fluorescence after 10 min. A sample with intermediate G6PD activity showed no or weak fluorescence after 5 min and moderate fluorescence after 10 min, while a deficient sample had very little or no fluorescence after 10 min. The FST test was performed along with normal, intermediate and deficient controls (Catalogue numbers G6888, G5029, and G5888, respectively, Trinity Biotech, Ireland). All results were read by two independent observers; when the interpretation of the readers was discordant, a third reader, blinded to the previous results was called in.

The CareStart G6PD deficiency RDT screening Kit (Catalogue number RGPM-02572) was used according to the manufacturer’s instructions. Briefly, 2 µL of whole blood were pipetted from the EDTA tube and added to the sample well followed by the addition of two drops of the assay buffer. All results were read after 10 min. Tests showing a distinct purple colour were interpreted as G6PD normal, tests showing no colour change, or a very faint purple colour were classified as deficient. Tests with no blood migration or incomplete blood migration were repeated. Tests were classified as invalid after failing to obtain a valid result in at least three attempts.

G6PD activity was measured by spectrophotometry in duplicate using the Trinity Biotech Assay (Kit no. 345-B; Trinity Biotech, Bray, Ireland). Normal, intermediate and deficient G6PD activity controls (Catalogue numbers G6888, G5029, and G5888, respectively) were run in duplicate at the beginning of each assay day. Sample testing was done if all three control values fell within a predefined activity range provided by the manufacturer. Duplicates for which the measurement values differed by more than 10% were rejected for the analysis and retested. For each measurement 10 μL whole blood or control were added to 1 mL G6PD assay solution and incubated at room temperature for 5 min. Then, 2 mL of G6PD substrate were added to the solution and mixed by inversion. One millilitre of the mixture was aliquoted into ultraviolet (UV)-transparent disposable cuvettes (Eppendorf UVette cells, Germany). A spectrophotometer (Shimadzu UV 1800 series, Shimadzu, Kyoto, Japan) was used to measure the change in absorbance at 340 nm over 5 min. Applying a formula provided by the manufacturer (Trinity) G6PD activity was calculated as U/dL and normalized by haemoglobin measurements performed on the same sample at the same time by a digital haemoglobin meter (Hemocue 201, Hemocue, Ängelholm, Sweden).

Analysis was done using STATA version 14.0. (StataCorp, USA) and Excel (Microsoft Corp, USA). Categorical data were compared using McNemar’s test for correlated proportions, the Chi squared test, or Fisher’s exact test as appropriate. Test performance was calculated using standard formula [32]. In Laos 100% G6PD activity was defined by calculating the adjusted male median (AMM) [28]. In Cambodia the study population was purposively selected and 100% G6PD activity was defined as 11.8 U/gHb based on previous studies [16, 21]. G6PD deficiency (G6PDd) was then defined as any result below 10, 30 or 70% of the AMM. The FST and G6PD RDT were evaluated considering spectrophotometry as the reference method. Areas under the receiver operating curve (ROC) were calculated for each assay applying 10, 30 and 70% cut-off activities and using the formula for binary tests [33], areas were subsequently compared for significant differences in size [34]. Analysis for the FST was done repeatedly, considering intermediate results (FSTdefint) either as G6PD deficient (FSTdef) or G6PD normal.

The AMM by spectrophotometry (AMM) in Laos was 11.5 U/gHb, with 1.5% (n = 11) of all participants having G6PD activities below 10% of the AMM, 5.2% (n = 28) between 10 and below 30% and 12.2% (n = 53) having activities between 30 and below 70% of the AMM. A total of three female participants had G6PD activities below 30% of the AMM, compared to 36 male participants (p < 0.001), whereas significantly more females (n = 37) than males (n = 16) had intermediate G6PD activities between 30 and 70% of the AMM (Fig. 1). In the non-randomly selected Cambodian population (n = 505), 100% G6PD activity was defined as 11.8 U/gHb [16, 21], with 8.7% (n = 44) of all participants having G6PD activities of less than 10, 20.0% (n = 101) having G6PD activities between 10% and less than 30% G6PD activity and 28.3% (n = 143) having G6PD activities between 30% and less than 70% G6PD activity. Significantly less females than males had G6PD activities below 30% (n = 36, p < 0.001), whereas significantly more females had intermediate G6PD activities between 30% and 70% (n = 103) compared to males (p < 0.001).

Sensitivity and specificity of the FST and the G6PD RDT compared to spectrophotometry are presented in Table 1. Both FST and RDT performed significantly better in Laos compared to Cambodia, irrespective of definition or cut-off applied (Table 1).