In biological systems, heme-copper oxidase (HCO) enzymes play a crucial role in the oxygen reduction reaction (ORR), where the pivotal O-O bond cleavage of the (heme)Fe-peroxo-Cu intermediate is facilitated by active-site (peroxo core) hydrogen bonding followed by proton-coupled electron transfer (PCET) from a nearby (phenolic) tyrosine residue. A useful approach to comprehend the fundamental relationships among H-bonding/proton/H-atom donors and their abilities to induce O-O bond homolysis involves the investigation of synthetic, bioinspired model systems where the exogenous substrate properties (such as p and bond dissociation energy (BDE)) can be systematically altered. This report details the reactivity of a heme-peroxo-copper HCO model complex (LS-4DCHIm) toward a series of substituted catechol substrates that span a range of p and O-H bond BDE values, exhibiting different reaction mechanisms. Considering their interactions with the bridging peroxo ligand in LS-4DCHIm, the catechol substrates are importantly capable of one or two (i) H-bonds, (ii) proton transfers, and/or (iii) net H-atom transfers, thereby making them attractive, yet complex candidates for studying the redox chemistry of the metal-bound peroxide. A combination of spectroscopic studies and kinetic analysis implies that the suitable modulation of p and O-H bond BDE values of catechols result in either double proton transfer with the release of HO or double PCET resulting in reductive O-O bond rupture. The distinguishing role of substrate properties in directing the mechanism and outcome of O protonation/reduction reactions is discussed in terms of designing O-reduction catalysts based on biological inspiration.

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http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11707526PMC
http://dx.doi.org/10.1039/d4sc05623jDOI Listing

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