Simultaneous Determination of A Novel Antitrypanosomal Compound (OSU-36) and its Ester Derivative (OSU-40) in Plasma by HPLC: Application to First Pharmacokinetic Study in Rats

Authors

  • Pavel Gershkovich University of British Columbia
  • Kishor M. Wasan
  • Olena Sivak
  • Summer Lysakowski
  • Carolyn Reid
  • Kokku Premalatha
  • Karl A. Werbovetz

DOI:

https://doi.org/10.18433/J3CP4S

Abstract

Purpose. To develop an HPLC-UV method for determination of a novel antitrypanosomal compound (OSU-36) and its ester prodrug (OSU-40) in rat plasma and to apply the method for pharmacokinetic evaluation of both compounds in rats. Methods. Since an attempt to assay for OSU-36 and OSU-40 in non-stabilized plasma resulted in highly non-linear calibration curves and poor sensitivity due to instability of the compounds, the plasma was stabilized using paraoxon and ascorbic acid. The sample treatment included protein precipitation by acetonitrile; evaporation; reconstitution with acetonitrile and filtration. The chromatography conditions included Xterra RP18 3.5µm 4.6X100mm column and gradient mobile phase system of acetonitrile-water. Results. The limits of quantification (LOQ) were 50 ng/mL and 40 ng/mL for OSU-36 and OSU-40, respectively. The intra- and interday precision and accuracies were below 13% for low, medium and high quality control samples for both compounds. While OSU-40 has been stable in all tested handling conditions, OSU-36 was unstable in plasma after 20 days storage in -80°C or 4h 28°C storage. The developed method has been applied for a pharmacokinetic study in rats which revealed that an ester prodrug OSU-40 is rapidly converted to OSU-36 within the plasma compartment by plasma esterases. OSU-36, in turn, relatively quickly undergoes oxidative metabolism, including within the plasma compartment. Conclusions. A supplementation of rat plasma with an esterase inhibitor to prevent degradation of ester prodrug (OSU-40), and with antioxidant to prevent oxidation of OSU-36, is necessary for reliable determination of both compounds. Due to limited stability of OSU-36 in stabilized rat plasma, long-term storage of samples or prolonged handling in room temperature conditions is not recommended.

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Author Biography

Pavel Gershkovich, University of British Columbia

Research Associate Faculty of Pharmaceutical Sciences

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Published

2011-01-30

How to Cite

Gershkovich, P., Wasan, K. M., Sivak, O., Lysakowski, S., Reid, C., Premalatha, K., & Werbovetz, K. A. (2011). Simultaneous Determination of A Novel Antitrypanosomal Compound (OSU-36) and its Ester Derivative (OSU-40) in Plasma by HPLC: Application to First Pharmacokinetic Study in Rats. Journal of Pharmacy & Pharmaceutical Sciences, 14(1), 36–45. https://doi.org/10.18433/J3CP4S

Issue

Vol. 14 No. 1 (2011)

Section

Pharmaceutical Sciences; Review Articles

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