4.8 Article

Reaction Coordinate of a Functional Model of Tyrosinase: Spectroscopic and Computational Characterization

Journal

JOURNAL OF THE AMERICAN CHEMICAL SOCIETY
Volume 131, Issue 18, Pages 6421-6438

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/ja807898h

Keywords

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Funding

  1. NIH [GM50730, DK31450]
  2. NSF [CNS-0619926]
  3. Theoretical and Computational Biophysics group at the Beckman Institute
  4. University of Illinois at Urbana-Champaign

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The mu-eta(2):eta(2)-peroxodicopper(II) complex synthesized by reacting the Cu(I) complex of the bisdiamine ligand N,N'-di-tert-butyl-ethylenediamine (DBED) with O-2 is a functional and spectroscopic model of the coupled binuclear copper protein tyrosinase. This complex reacts with 2,4-di-tert-butylphenolate at low temperature to produce a mixture of the catechol and quinone products, which proceeds through three intermediates (A-C) that have been characterized. A, stabilized at 153 K, is characterized as a phenolate-bonded bis-mu-oxo dicopper(III) species, which proceeds at 193 K to B, presumably a catecholate-bridged coupled bis-copper(II) species via an electrophilic aromatic substitution mechanism wherein aromatic ring distortion is the rate-limiting step. Isotopic labeling shows that the oxygen inserted into the aromatic substrate during hydroxylation derives from dioxygen, and a late-stage ortho-H+ transfer to an exogenous base is associated with C-O bond formation. Addition of a proton to B produces C, determined from resonance Raman spectra to be a Cu(II)-semiquinone complex. The formation of C (the oxidation of catecholate and reduction to Cu(I)) is governed by the protonation state of the distal bridging oxygen ligand of B. Parallels and contrasts are drawn between the spectroscopically and computationally supported mechanism of the DBED system, presented here, and the experimentally derived mechanism of the coupled binuclear copper protein tyrosinase.

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