Gp. Mcmahon et al., HIGH-PERFORMANCE LIQUID-CHROMATOGRAPHIC DETERMINATION OF TAURINE IN HUMAN PLASMA USING PRECOLUMN EXTRACTION AND DERIVATIZATION, Journal of pharmaceutical and biomedical analysis, 14(8-10), 1996, pp. 1287-1294
Plasma samples (100 mu l) were treated with 150 mu l of acetonitrile a
nd centrifuged at 5800g for 10 min and 50 mu l of 10 mM berate buffer
(pH 9.2) were added to the supernatant solution. This was followed by
the addition of a 50 mu l aliquot of 5 mM fluorescamine in acetonitril
e and immediate vortex mixing. A 20 mu l sample was injected on to a r
eversed-phase HPLC system using a Bondclone C-18 10 mu m analytical co
lumn (300 mm x 3.9 mm). The mobile phase was tetrahydrofuran-acetonitr
ile-phosphate buffer (15 mM, pH 3.5) (4:24:72, v/v/v). The taurine der
ivative was detected by measuring the UV absorbance of 385 nm. Platele
t-poor plasma samples were spiked with known amounts of taurine and in
ter- and intra-assay calibration curves were obtained. The method was
applied to the determination of taurine in platelet-rich plasma.