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Vol. 63, Issue 1, 136-146, January 2003
Department of Pharmacology and Toxicology, Faculty of Health
Sciences, Queen's University, Kingston, Ontario, Canada
Peroxynitrite (ONOO
) toxicity is associated with protein
oxidation and/or tyrosine nitration, usually resulting in inhibition of
enzyme activity. We examined the effect of ONOO
on the
activity of purified rat liver microsomal glutathione S-transferase (GST) and found that the activity of
reduced glutathione (GSH)-free enzyme was increased 4- to 5-fold by 2 mM ONOO
; only 15% of this increased activity was
reversed by dithiothreitol. Exposure of the microsomal GST to
ONOO
resulted in concentration-dependent oxidation of
protein sulfhydryl groups, dimer and trimer formation, protein
fragmentation, and tyrosine nitration. With the exception of sulfhydryl
oxidation, these modifications of the enzyme correlated well with the
increase in enzyme activity. Nitration or acetylation of tyrosine
residues of the enzyme using tetranitromethane and
N-acetylimidazole, respectively, also resulted in
increased enzyme activity, providing additional evidence that
modification of tyrosine residues can alter catalytic activity.
Addition of ONOO
-treated microsomal GST to microsomal
membrane preparations caused a marked reduction in iron-induced lipid
peroxidation, which raises the possibility that this enzyme may act to
lessen the degree of membrane damage that would otherwise occur under
pathophysiological conditions of increased ONOO
formation.
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