Oxidation of tryptophan by redox intermediates of myeloperoxidase and inhibition of hypochlorous acid production

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Abstract

The neutrophil enzyme myeloperoxidase catalyzes the oxidation of tyrosine to tyrosyl radicals, which cross-link to proteins and initiate lipid peroxidation. Tryptophan is present in plasma at about the same concentration as tyrosine and has a similar one-electron reduction potential. In this investigation, we have determined the ability of myeloperoxidase to catalyze the oxidation of tryptophan to assess whether or not this reaction may contribute to oxidative stress at sites of inflammation. We show that tryptophan is a poor substrate for myeloperoxidase because, even though it reacts rapidly with compound I (k1 2.1 x 106 M 1s 1), it reacts sluggishly with compound II (k11 7 M-1s-1). Tryptophan reversibly inhibited production of hypochlorous acid by purified myeloperoxidase by converting the enzyme to a mixture of compound II and compound III. It gave 50% inhibition (I50) at a concentration of 2 μM. In contrast, it was an ineffective inhibitor of hypochlorous acid production by human neutrophils (I50 80 μM) unless superoxide dismutase was present (I50 5 μM). We propose that compound I of myeloperoxidase will oxidize tryptophan at sites of inflammation. Enzyme turnover will result from the reaction of superoxide or tyrosine with compound II. Thus, tryptophan radicals are potential candidates for exacerbating oxidative stress during inflammation.

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Kettle, A. J., & Candaeis, L. P. (2000). Oxidation of tryptophan by redox intermediates of myeloperoxidase and inhibition of hypochlorous acid production. Redox Report, 5(4), 179–184. https://doi.org/10.1179/135100000101535726

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