Nitration and inactivation of cytochrome P450BMâ3 by peroxynitrite: Stoppedâflow measurements prove ferryl intermediates
2000
Daiber, Andreas | Herold, Susanna | Schöneich, Christian | Namgaladze, Dmitry | Peterson, Julian A. | Ullrich, Volker
Peroxynitrite (PN) is likely to be generated in vivo from nitric oxide and superoxide. We have previously shown that prostacyclin synthase, a hemeâthiolate enzyme essential for regulation of vascular tone, is nitrated and inactivated by submicromolar concentrations of PN [Zou, M.âH. & Ullrich, V. (1996) FEBS Lett.382, 101–104] and we have studied the effect of heme proteins on the PNâmediated nitration of phenolic compounds in model systems [Mehl, M., Daiber, A. & Ullrich, V. (1999) Nitric Oxide: Biol. Chem.2, 259–269]. In the present work we show that bolus additions of PN or PNâgenerating systems, such as SINâ1, can induce the nitration of P450BMâ3 (wildâtype and F87Y variant), for which we suggest an autocatalytic mechanism. HPLC and MSâanalysis revealed that the wildâtype protein is selectively nitrated at Y334, which was found at the entrance of a water channel connected to the active site iron center. In the F87Y variant, Y87, which is directly located at the active site, was nitrated in addition to Y334. According to Western blots stained with a nitrotyrosine antibody, this nitration started at 0.5âµm of PN and was halfâmaximal between 100 and 150âµm of PN. Furthermore, PN caused inactivation of the P450BMâ3 monooxygenase as well as the reductase activity with an IC50 value of 2–3âµm. As two thiol residues/protein molecule were oxidized by PN and the inactivation was prevented by GSH or dithiothreitol, but not by uric acid (a powerful inhibitor of the nitration), our data strongly indicate that the inactivation is due to thiol oxidation at the reductase domain rather then to nitration of Y residues. Stoppedâflow data presented here support our previous hypothesis that ferrylâspecies are involved as intermediates during the reactions of P450 enzymes with PN.
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