INVESTIGADORES
GOICOECHEA Hector Casimiro
artículos
Título:
Simultaneous determination of naphazoline, diphenhydramine and phenilephrine in nasal solutions by capillary electrophoresis
Autor/es:
A MARCHESINI,; M WILINER,; V MANTOVANI,; JC ROBLES,; GOICOECHEA, HÉCTOR C
Revista:
JOURNAL OF PHARMACEUTICAL AND BIOMEDICAL ANALYSIS
Editorial:
Elsevier
Referencias:
Año: 2003 vol. 31 p. 39 - 46
ISSN:
0731-7085
Resumen:
A capillary zone electrophoresis (CZE) method has been developed to separate and quantitate naphazoline (NAPH),
dyphenhydramine (DIP) and phenylephrine (PHE) in nasal solutions. Samples were diluted 1:25 in ultrapure water and
injected at the anodic end. A central composite design has been used to optimise the experimental conditions for a
complete and fast separation of the active ingredients studied. Critical parameters such as voltage, pH and buffer
concentration have been studied to evaluate how they affect responses such as resolution and migration times.
Separation was performed on a silica capillary with 75 mm I.D. and 70 cm total length at an applied voltage of 17.7 kV
with a phosphate run buffer of pH 3.72 and 0.063 mol l1. Calibration curves were prepared for NAPH, DIP and PHE.
For each analyte, the correlation coefficients were /0.999 (n/15). The RSD% of six replicate injections for each
analyte were reasonably good. The method was applied to the quantitation of the three components in a commercial
dosage form. The proposed method has the advantage of needing a very simple sample pretreatment and being faster
than a typical HPLC chromatographic method.veloped to separate and quantitate naphazoline (NAPH),
dyphenhydramine (DIP) and phenylephrine (PHE) in nasal solutions. Samples were diluted 1:25 in ultrapure water and
injected at the anodic end. A central composite design has been used to optimise the experimental conditions for a
complete and fast separation of the active ingredients studied. Critical parameters such as voltage, pH and buffer
concentration have been studied to evaluate how they affect responses such as resolution and migration times.
Separation was performed on a silica capillary with 75 mm I.D. and 70 cm total length at an applied voltage of 17.7 kV
with a phosphate run buffer of pH 3.72 and 0.063 mol l1. Calibration curves were prepared for NAPH, DIP and PHE.
For each analyte, the correlation coefficients were /0.999 (n/15). The RSD% of six replicate injections for each
analyte were reasonably good. The method was applied to the quantitation of the three components in a commercial
dosage form. The proposed method has the advantage of needing a very simple sample pretreatment and being faster
than a typical HPLC chromatographic method.ve ingredients studied. Critical parameters such as voltage, pH and buffer
concentration have been studied to evaluate how they affect responses such as resolution and migration times.
Separation was performed on a silica capillary with 75 mm I.D. and 70 cm total length at an applied voltage of 17.7 kV
with a phosphate run buffer of pH 3.72 and 0.063 mol l1. Calibration curves were prepared for NAPH, DIP and PHE.
For each analyte, the correlation coefficients were /0.999 (n/15). The RSD% of six replicate injections for each
analyte were reasonably good. The method was applied to the quantitation of the three components in a commercial
dosage form. The proposed method has the advantage of needing a very simple sample pretreatment and being faster
than a typical HPLC chromatographic method.ve been studied to evaluate how they affect responses such as resolution and migration times.
Separation was performed on a silica capillary with 75 mm I.D. and 70 cm total length at an applied voltage of 17.7 kV
with a phosphate run buffer of pH 3.72 and 0.063 mol l1. Calibration curves were prepared for NAPH, DIP and PHE.
For each analyte, the correlation coefficients were /0.999 (n/15). The RSD% of six replicate injections for each
analyte were reasonably good. The method was applied to the quantitation of the three components in a commercial
dosage form. The proposed method has the advantage of needing a very simple sample pretreatment and being faster
than a typical HPLC chromatographic method.mm I.D. and 70 cm total length at an applied voltage of 17.7 kV
with a phosphate run buffer of pH 3.72 and 0.063 mol l1. Calibration curves were prepared for NAPH, DIP and PHE.
For each analyte, the correlation coefficients were /0.999 (n/15). The RSD% of six replicate injections for each
analyte were reasonably good. The method was applied to the quantitation of the three components in a commercial
dosage form. The proposed method has the advantage of needing a very simple sample pretreatment and being faster
than a typical HPLC chromatographic method.1. Calibration curves were prepared for NAPH, DIP and PHE.
For each analyte, the correlation coefficients were /0.999 (n/15). The RSD% of six replicate injections for each
analyte were reasonably good. The method was applied to the quantitation of the three components in a commercial
dosage form. The proposed method has the advantage of needing a very simple sample pretreatment and being faster
than a typical HPLC chromatographic method./0.999 (n/15). The RSD% of six replicate injections for each
analyte were reasonably good. The method was applied to the quantitation of the three components in a commercial
dosage form. The proposed method has the advantage of needing a very simple sample pretreatment and being faster
than a typical HPLC chromatographic method.vantage of needing a very simple sample pretreatment and being faster
than a typical HPLC chromatographic method.