EDTA analysis on the Roche MODULAR® analyser

Background Patient specimens can be subject to subtle interference from cross contamination by liquid-based, potassium-containing EDTA anticoagulant, leading to misinterpretation of results. A rapid method for EDTA analysis to detect such contamination is described. Method An in-house EDTA assay on the Roche MODULAR (R) analyser was assessed for accuracy and precision by comparison with an adjusted calcium difference measurement (atomic absorption and o-cresolphthalein complexone colorimetry). Results EDTA method versus adjusted calcium difference showed: slope = 1.038 (95% confidence interval [CI] 0.949-1.131); intercept = 0.073 (95% Cl 0.018-0.132) mmol/L; r== 0.914; n = 94. However, inter-assay precision of the calcium difference method was estimated to be poorer (coefficient of variation 24.8% versus 3.4% for the automated colorimetric method at an EDTA concentration of 0.25 mmol/Q. Unequivocal contamination was observed at an EDTA concentration of >, 0.2 mmol/L. The automated method showed positive interference from haemolysis and negative interference from oxalate. The method was unaffected by lipaemia (triglycerides < 20 mmol/L), icterus (bilirubin < 500,umol/L), glucose (< 100 mmol/L), iron (< 1 00,umol/L), and citrate, phosphate or fluoride (all < 2.5 mmol/L). Conclusion The automated colorimetric assay described is an accurate, precise and rapid (3 min) means of detecting EDTA contamination of unhaemolysed biochemistry specimens.