Development and Validation of Atorvastatin by LC-ESI-MS and Application in Bioequivalence Research in Healthy Chinese Volunteers
The aim of this research was to develop a sensitive liquid chromatographic-electrospray ionization-mass spectrometric (LC-MS) method for direct measurement of the concentration of Atorvastatin in human plasma. Plasma samples (1 mL) were extracted with 3 mL ethyl acetate, and by a simple reversed-pha...
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Published in | Chromatographia Vol. 65; no. 11-12; pp. 737 - 741 |
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Main Authors | , , , |
Format | Journal Article |
Language | English |
Published |
Oxford
Wiesbaden : Vieweg Verlag
01.06.2007
Springer Springer Nature B.V |
Subjects | |
Online Access | Get full text |
ISSN | 0009-5893 1612-1112 |
DOI | 10.1365/s10337-007-0236-4 |
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Abstract | The aim of this research was to develop a sensitive liquid chromatographic-electrospray ionization-mass spectrometric (LC-MS) method for direct measurement of the concentration of Atorvastatin in human plasma. Plasma samples (1 mL) were extracted with 3 mL ethyl acetate, and by a simple reversed-phase chromatography. Pitavastatin was used as internal standard (IS). The LOQ was 0.25 ng mL-¹ (RSD 4.24%). The assay was linear from 0.25-20 ng mL-¹. And the correlation coefficient for the calibration regression line was 0.9996 or better. Intra-day and inter-day accuracy were better than 15%. The method has been successfully used for a pharmacokinetic study with human subjects. A two-period crossover designed bioequivalence research was also progressed in healthy Chinese volunteers. Among the pharmacokinetic data obtained, T max was 1.36 ± 0.68 h for reference formulation and 0.81 ± 0.54 h for test formulation. C max was 8.54 ± 5.06 ng mL-¹ for reference formulation and 9.54 ± 3.68 ng mL-¹ for test formulation. t ₁/₂ was 8.50 ± 2.74 h for reference formulation and 9.24 ± 3.17 h for test formulation. AUC ₀-₄₈h was 54.77 ± 21.82 h ng mL-¹ for reference formulation and 55.66 ± 20.91 h ng mL-¹ for test formulation. The method was successfully applied to the study of pharmacokinetics of Atorvastatin in healthy Chinese volunteers. |
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AbstractList | The aim of this research was to develop a sensitive liquid chromatographic–electrospray ionization–mass spectrometric (LC–MS) method for direct measurement of the concentration of Atorvastatin in human plasma. Plasma samples (1 mL) were extracted with 3 mL ethyl acetate, and by a simple reversed-phase chromatography. Pitavastatin was used as internal standard (IS). The LOQ was 0.25 ng mL−1 (RSD 4.24%). The assay was linear from 0.25–20 ng mL−1. And the correlation coefficient for the calibration regression line was 0.9996 or better. Intra-day and inter-day accuracy were better than 15%. The method has been successfully used for a pharmacokinetic study with human subjects. A two-period crossover designed bioequivalence research was also progressed in healthy Chinese volunteers. Among the pharmacokinetic data obtained, Tmax was 1.36 ± 0.68 h for reference formulation and 0.81 ± 0.54 h for test formulation. Cmax was 8.54 ± 5.06 ng mL−1 for reference formulation and 9.54 ± 3.68 ng mL−1 for test formulation. t1/2 was 8.50 ± 2.74 h for reference formulation and 9.24 ± 3.17 h for test formulation. AUC0−48h was 54.77 ± 21.82 h ng mL−1 for reference formulation and 55.66 ± 20.91 h ng mL−1 for test formulation. The method was successfully applied to the study of pharmacokinetics of Atorvastatin in healthy Chinese volunteers. The aim of this research was to develop a sensitive liquid chromatographic-electrospray ionization-mass spectrometric (LC-MS) method for direct measurement of the concentration of Atorvastatin in human plasma. Plasma samples (1 mL) were extracted with 3 mL ethyl acetate, and by a simple reversed-phase chromatography. Pitavastatin was used as internal standard (IS). The LOQ was 0.25 ng mL-¹ (RSD 4.24%). The assay was linear from 0.25-20 ng mL-¹. And the correlation coefficient for the calibration regression line was 0.9996 or better. Intra-day and inter-day accuracy were better than 15%. The method has been successfully used for a pharmacokinetic study with human subjects. A two-period crossover designed bioequivalence research was also progressed in healthy Chinese volunteers. Among the pharmacokinetic data obtained, T max was 1.36 ± 0.68 h for reference formulation and 0.81 ± 0.54 h for test formulation. C max was 8.54 ± 5.06 ng mL-¹ for reference formulation and 9.54 ± 3.68 ng mL-¹ for test formulation. t ₁/₂ was 8.50 ± 2.74 h for reference formulation and 9.24 ± 3.17 h for test formulation. AUC ₀-₄₈h was 54.77 ± 21.82 h ng mL-¹ for reference formulation and 55.66 ± 20.91 h ng mL-¹ for test formulation. The method was successfully applied to the study of pharmacokinetics of Atorvastatin in healthy Chinese volunteers. |
Author | Chen, X. J Ma, L Dong, J Wang, G. J |
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Keywords | Human Validation Column liquid chromatography Chemical analysis Bioequivalence LC-ESI-MS Enzyme Coupled method Volunteer Oral administration Enzyme inhibitor HPLC chromatography Statin derivative Normal Electrospray Reversed phase chromatography Atorvastatin Hydroxymethylglutaryl-CoA reductase Oxidoreductases Pharmacokinetics Mass spectrometry Quantitative analysis Antilipemic agent |
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SubjectTerms | Analysis Atorvastatin Bioequivalence Biological and medical sciences Blood plasma Correlation coefficients electrospray ionization mass spectrometry Ethyl acetate General pharmacology humans LC-ESI-MS liquid chromatography Medical sciences Pharmacokinetics Pharmacology Pharmacology. Drug treatments reversed-phase liquid chromatography Spectrometry volunteers |
Title | Development and Validation of Atorvastatin by LC-ESI-MS and Application in Bioequivalence Research in Healthy Chinese Volunteers |
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