Simultaneous determination of melatonin–pyridoxine combination in tablets by zero-crossing derivative spectrophotometry and spectrofluorimetry
Journal of pharmaceutical and biomedical analysis, 1998•Elsevier
Two methods have been developed for the analysis of melatonin (M) and pyridoxine
hydrochloride (PH) in combination. The first method depends on first-and second-derivative
ultraviolet spectrophotometry, with the zero crossing technique of measurement. First-
derivative amplitudes at 296 nm and second-derivative amplitudes at 294 and 322 nm are
selected for the determination of M and PH, respectively. The second method is based on
the native fluorescence of both M and PH, in methanol and 0.1 M hydrochloric acid …
hydrochloride (PH) in combination. The first method depends on first-and second-derivative
ultraviolet spectrophotometry, with the zero crossing technique of measurement. First-
derivative amplitudes at 296 nm and second-derivative amplitudes at 294 and 322 nm are
selected for the determination of M and PH, respectively. The second method is based on
the native fluorescence of both M and PH, in methanol and 0.1 M hydrochloric acid …
Two methods have been developed for the analysis of melatonin (M) and pyridoxine hydrochloride (PH) in combination. The first method depends on first- and second-derivative ultraviolet spectrophotometry, with the zero crossing technique of measurement. First-derivative amplitudes at 296 nm and second-derivative amplitudes at 294 and 322 nm are selected for the determination of M and PH, respectively. The second method is based on the native fluorescence of both M and PH, in methanol and 0.1 M hydrochloric acid, respectively, after a preliminary solvent extraction procedure. The relative standard deviation of both methods was less than 2.0%. The two methods have been successfully applied to the determination of both drugs in laboratory-prepared mixtures and in tablets
Elsevier
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