A novel colorimetric assay for the determination of lysophosphatidic acid in plasma using an enzymatic cycling method

Abstract Background : Several methods for measuring concentrations of lysophosphatidic acid (LPA), a lipid mediator, have been reported to date. However, these methods are not routinely used because most of them require specialized instrument and a complicated protocol. Methods : We developed a novel LPA assay using enzymatic cycling. LPA in a sample is hydrolyzed with lysophospholipase to glycerol-3-phosphate, followed by enzymatic cycling using glycerol-3-phosphate oxidase and glycerol-3-phosphate dehydrogenase. Amplified concentrations of hydrogen peroxides, a product of the enzymatic cycling, are then colorimetrically measured. Results : This method was specific for LPA, being insensitive to the presence of phosphatidic acid or lysophosphatidylcholine. The within-run and between-run CVs were 1.31–1.32% and 0.73–1.03%, respectively. The recoveries of exogenous LPA added to plasma were 100.3–101.6%. In males, LPA concentrations (mean±S.D.) of human serum and EDTA-plasma were 0.41±0.14 and 0.08±0.02 μmol/l, respectively. In females, they were 0.41±0.12 and 0.09±0.02 μmol/l, respectively. Conclusions : This novel colorimetric assay for determination of LPA using enzymatic cycling is simple and highly sensitive. It can be used with an automatic analyzer. It may also be useful for further studies of the biological functions of LPA as well as clinical applications in various disorders.