Nantana NuchtavornLeena SuntornsukMahidol University2018-06-112018-06-112012-02-01Journal of Chromatographic Science. Vol.50, No.2 (2012), 151-156002196652-s2.0-84858844150https://repository.li.mahidol.ac.th/handle/20.500.14594/13986A capillary zone electrophoretic method using UV detection is developed for the analysis of four biological active pyridines [i.e., nicotine (NIC), cotinine (COT), nicotinic acid (NA), and nicotinamide (NM)]. The separation of the pyridines is achieved in 25 mM sodium dihydrogen phosphate (pH 2.1) using a fused-silica capillary with an effective length of 56 cm and an inner diameter of 50 m (extended light path), hydrodynamic injection at 50 mbar for 10 s, a temperature of 25°C, applied voltage of 30 kV, and UV detection at 260 nm. These conditions provide baseline separation of all the analytes [resolution (Rs) > 3.6] in 9.4 min with good linearity (r 2 > 0.998, in ranges of 50600 g/mL for NIC, 8160 g/mL for NM, and 10200 g/mL for COT and NA), precision (relative standard deviation < 2.04), recovery (96.4101.6), limits of detection ( < 3.0 g/mL), and quantitation ( < 10 g/mL). The method is robust upon the alterations of pH of BGE, separating voltage, and injection time [the RSDs of the relative migration time (migration time of the analyte/migration time of the internal standard) and resolution < 3.26]. The method is efficient, reliable, and simple for the routine analysis of NIC, NA, and NM in various products such as gum and tablets and can be applied to determine COT in thermal degradation of NIC gum. © 2012 The Author.Mahidol UniversityChemistryArticleSCOPUS10.1093/chromsci/bmr037