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Vol. 31, Issue 1, 76-87, January 2003
Departments of Pharmacokinetics, Dynamics, and Metabolism (K.J.,
S.J., J.B., C.P.) and Clinical Sciences (A.S.), Pfizer Global Research
and Development, Groton, Connecticut
The excretion, biotransformation, and pharmacokinetics of a
selective N-methyl-D-aspartate
receptor antagonist, traxoprodil, were investigated in six healthy male
volunteers, phenotyped either as CYP2D6 extensive or poor metabolizers
of dextromethorphan. Each subject received an i.v. infusion of a single
50-mg (100 µCi) dose of [14C]traxoprodil.
Approximately 89% of the administered dose was recovered in poor
metabolizers (PMs) and 61% in extensive metabolizers (EMs), with the
majority of the dose being excreted in the urine (86% in PMs and 52%
in EMs). The elimination of traxoprodil was more rapid in EMs than in
PMs with terminal elimination half-lives of 2.8 and 26.9 h,
respectively, for EMs and PMs. Area under the plasma concentration-time
curve from time 0 to T (AUC(0-Tlast)) values for unchanged
traxoprodil were 1.2 and 32.7% of the corresponding AUC values for
total radioactivity in EMs and PMs, respectively. Traxoprodil was
metabolized in both EMs and PMs, with ~7 and 50% of the administered
radioactivity excreted as unchanged drug in the excreta of EMs and PMs,
respectively. Hydroxylation at the 3-position of the hydroxyphenyl ring
and methylation of the resulting catechol followed by conjugation were
identified as the main metabolic pathways in EMs. In contrast,
direct conjugation of traxoprodil with glucuronic or sulfuric acid was
the major pathway in PMs. In vitro studies using CYP2D6-selective
inhibitor and recombinant enzyme also support that the metabolism of
traxoprodil is mainly mediated by CYP2D6. Taken together, these studies
suggest that traxoprodil is eliminated mainly by Phase I oxidative
metabolism mediated by CYP2D6 isozyme in EMs and by Phase II
conjugation and renal clearance of parent in PMs.
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