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Simultaneous evaluation of losartan and amlodipine besylate using second-derivative synchronous spectrofluorimetric technique and liquid chromatography with time-programmed fluorimetric detection
Author(s) -
Shereen Shalan,
Jenny Jeehan Nasr
Publication year - 2019
Publication title -
royal society open science
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.84
H-Index - 51
ISSN - 2054-5703
DOI - 10.1098/rsos.190310
Subject(s) - amlodipine , losartan , chromatography , derivative (finance) , chemistry , fluorescence , angiotensin ii , physics , biochemistry , receptor , biology , quantum mechanics , blood pressure , financial economics , economics , endocrinology
This study is concerned with two sensitive, fast and reproducible approaches; namely, second-derivative synchronous fluorimetry (method I) and reversed phase high-performance liquid chromatography with fluorimetric detection (method II) for synchronized evaluation of losartan (LOS) and amlodipine besylate (AML). Method I is based on measuring second-derivative synchronous fluorescence spectra of LOS and AML at Δ λ = 80 nm in water. The experimental factors influencing the synchronous fluorescence of the considered compounds were sensibly adjusted. The chromatographic analysis was executed on a Nucleodur MN-C18 column of dimensions; 250 × 4.6 mm i.d. and 5 µm particle size). The fluorimetric detection was time-programmed at λ em = 440 nm for AML (0.0–7.5 min) and at λ em = 400 nm for LOS (7.5–10 min) after excitation at λ ex = 245 nm. The mobile phase is a blend of acetonitrile with 0.02 M phosphate buffer in a proportion of 45 : 55, pH 4.0, pumped using a flow rate of 1 ml min −1 . The calibration plots were established to be 0.1–4.0 µg ml −1 for both drugs in method I and 0.05–4.0 µg ml −1 for both drugs in method II. The study was extended to the evaluation of the two drugs in their co-formulated tablets.

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