1. Academic Validation
  2. Species differences in the pharmacokinetics and metabolism of reparixin in rat and dog

Species differences in the pharmacokinetics and metabolism of reparixin in rat and dog

  • Xenobiotica. 2006 May;36(5):419-40. doi: 10.1080/00498250600646517.
I Midgley 1 K Fitzpatrick S J Wright B A John A J Peard R M Major J D Holding A McBurney R Anacardio R Novellini M P Ferrari
Affiliations

Affiliation

  • 1 Department of Drug Metabolism, Huntingdon Life Sciences Ltd, Huntingdon, UK. MidgleyI@ukorg.Huntingdon.com
Abstract

The pharmacokinetics and metabolism of reparixin (formerly repertaxin), a potent and specific inhibitor of the chemokine CXCL8, were investigated in rats and dogs after intravenous administration of [14C]-reparixin L-lysine salt. Protein binding of reparixin was investigated in vitro in rat, dog, rabbit, cynomolgus monkey and human plasma. Plasma protein binding of reparixin was >99% in the laboratory Animals and humans up to 50 microg ml-1, but lower at higher concentrations. Although radioactivity was rapidly distributed into rat tissues, Vss was low (about 0.15 l kg-1) in both rat and dog. Nevertheless, reparixin was more rapidly eliminated in rats (t1/2 approximately 0.5 h) than in dogs (t1/2 approximately 10 h). Systemic exposure in dog was due primarily to parent drug, but metabolites played a more prominent role in rat. Oxidation of the isobutyl side-chain was the major metabolic pathway in rat, whereas hydrolysis of the amide bond predominated in dog. Urinary excretion, which accounted for 80-82% of the radioactive dose, was the major route of elimination in both species, and biotransformation of reparixin was complete before excretion.

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