A liquid chromatographic method with a rapid clean-up procedure was used for the determination of caffeine in rat plasma and brain tissue after administration of a single dose of caffeine (2mg/kg, iv). Plasma and brain tissue homogenates were deproteinated by acetonitrile and then centrifuged. Separation was achieved on a Cosmosile C18 column with a mobile phase of 0.1 M borate buffer (pH 6.4)-methanol (72:28, v/v). The limit of detection of caffeine was 0.01μg/mL. The results suggest that the plasma concentration versus time profile of caffeine fits a two-compartment open model, and that the elimination half-life of caffeine is 77.2±4.4min in rat blood. Fifteen mm after caffeine administration, there were no significant differences in caffeine concentration among various regions of the rat brain (cerebral cortex, cerebellum, hippocampus, brain stem, striatum and midbrain).