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Vol. 54, Issue 2, 445-451, August 1998
Institute of Pharmaceutical Chemistry, University of Frankfurt,
D-60439 Frankfurt, Germany
Nonredox type 5-lipoxygenase (5-LO) inhibitors, such as ZM 230487, its
methyl analogue ZD 2138, or the Merck compound L-739,010, suppress
cellular leukotriene synthesis of ionophore stimulated granulocytes
with IC50 values of about 50 nM. However, in
cell homogenates or in preparations of purified enzyme, up to 150-fold higher concentrations are required for similar inhibition of 5-LO activity. This loss of 5-LO inhibition in cell homogenates was reversed
by addition of glutathione or dithiothreitol, which increased the
inhibitory potency of ZM 230487 or L-739,010 by about 100 to 150-fold
so that 5-LO inhibition was comparable with that of intact cells. In
the presence of thiols, addition of hydroperoxide [13(S)-HpODE], glutathione-peroxidase inhibition by
iodacetate or selenium-deficiency lead to impaired 5-LO
inhibition by ZM 230487 in cell homogenates. Moreover, addition of
glutathione peroxidase was required for efficient inhibition of
purified human 5-LO by ZM 230487. The data suggest that low
hydroperoxide concentrations are important for efficient 5-LO
inhibition by ZM 230487. The kinetic analysis revealed a noncompetitive
inhibition of 5-LO by ZM 230487 at low hydroperoxide levels, whereas it
acted as a competitive inhibitor with low affinity under nonreducing
conditions in granulocyte homogenates. No such redox-dependent effects
were observed with the 5-LO inhibitor BWA4C, the 5-LO activating
protein-inhibitor MK-886 or the pentacyclic triterpene
acetyl-11-keto-
-boswellic acid. These data suggest that
physiological conditions associated with oxidative stress and increased
peroxide levels lead to impaired efficacy of nonredox type 5-LO
inhibitors like ZM 230487 or L-739,010. This could explain the reported
lack of activity of this class of 5-LO inhibitors in chronic
inflammatory processes.
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