Determination of nimodipine in plasma by HPLC-MS/MS and pharmacokinetic application

Authors

  • Demétrius Fernandes do Nascimento Federal University of Ceará; Department of Physiology and Pharmacology
  • Manoel Odorico de Moraes Federal University of Ceará; Department of Physiology and Pharmacology
  • Fernando Antônio Frota Bezerra Federal University of Ceará; Department of Physiology and Pharmacology
  • Andréa Vieira Pontes Federal University of Ceará; Department of Physiology and Pharmacology
  • Célia Regina Amaral Uchoa Federal University of Ceará; Department of Physiology and Pharmacology
  • Renata Amaral de Moraes Federal University of Ceará; Department of Physiology and Pharmacology
  • Ismenia Osório Leite Federal University of Ceará; Department of Physiology and Pharmacology
  • Gilmara Silva de Melo Santana Federal University of Ceará; Department of Physiology and Pharmacology
  • Ana Paula Macedo Santana Federal University of Ceará; Department of Physiology and Pharmacology
  • Ana Lourdes Almeida e Silva Leite Federal University of Ceará; Department of Physiology and Pharmacology
  • José Pedrazzoli Júnior Federal University of Ceará; Department of Physiology and Pharmacology
  • Maria Elisabete Amaral de Moraes Federal University of Ceará; Department of Physiology and Pharmacology

DOI:

https://doi.org/10.1590/S1984-82502010000400008

Keywords:

Nimodipine^i1^sdetermination in pla, Nimodipine^i1^spharmacokinetic prof, Nimodipine^i1^squantitative analy, Pharmacokinetics^i1^smethod validat

Abstract

To develop and validate a rapid, specific and highly sensitive method to quantify nimodipine in human plasma using dibucaine as the internal standard (IS). The analyte and IS were extracted from plasma samples by liquid-liquid extraction using hexane-ethyl acetate (1:1 v/v). The chromatographic separation was performed on a Varian® Polaris C18 analytical column (3 μm, 50 x 2.0 mm) and pre-column SecurityguardTM C18 (4.0 x 3.0 mm) with a mobile phase of Acetonitrile-Ammonium acetate 0.02 ml/L (80:20v/v). The method had a chromatographic run time of 4.5 min and linear calibration curve over the range of 0.1- 40 ng/mL (r >; 0.9938). The limit of quantification was 100 pg/mL. Acceptable precision and accuracy were obtained for concentrations over the standard curve ranges. This validated method was successfully applied in determining the pharmacokinetic profile of nimodipine tablets of 30 mg administered to 24 healthy volunteers. The proposed method of analysis provided a sensitive and specific assay for nimodipine determination in human plasma. The time for the determination of one plasma sample was 4.5 min. This method is suitable for the analysis of nimodipine in human plasma samples collected for pharmacokinetic, bioavailability or bioequivalence studies in humans.

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Published

2010-12-01

Issue

Vol. 46 No. 4 (2010)

Section

Articles

License

All content of the journal, except where identified, is licensed under a Creative Commons attribution-type BY.

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How to Cite

Determination of nimodipine in plasma by HPLC-MS/MS and pharmacokinetic application . (2010). Brazilian Journal of Pharmaceutical Sciences, 46(4), 665-677. https://doi.org/10.1590/S1984-82502010000400008