Abstract
Mononuclear Mo-containing enzymes of the xanthine oxidase (XO) family catalyze the oxidative hydroxylation of aldehydes and heterocyclic compounds. The molybdenum active site shows a distorted square-pyramidal geometry in which two ligands, a hydroxyl/water molecule (the catalytic labile site) and a sulfido ligand, have been shown to be essential for catalysis. The XO family member aldehyde oxidoreductase from Desulfovibrio gigas (DgAOR) is an exception as presents in its catalytically competent form an equatorial oxo ligand instead of the sulfido ligand. Despite this structural difference, inactive samples of DgAOR can be activated upon incubation with dithionite plus sulfide, a procedure similar to that used for activation of desulfo-XO. The fact that DgAOR does not need a sulfido ligand for catalysis indicates that the process leading to the activation of inactive DgAOR samples is different to that of desulfo-XO. We now report a combined kinetic and X-ray crystallographic study to unveil the enzyme modification responsible for the inactivation and the chemistry that occurs at the Mo site when DgAOR is activated. In contrast to XO, which is activated by resulfuration of the Mo site, DgAOR activation/inactivation is governed by the oxidation state of the dithiolene moiety of the pyranopterin cofactor, which demonstrates the non-innocent behavior of the pyranopterin in enzyme activity. We also showed that DgAOR incubation with dithionite plus sulfide in the presence of dioxygen produces hydrogen peroxide not associated with the enzyme activation. The peroxide molecule coordinates to molybdenum in a η2 fashion inhibiting the enzyme activity.
Highlights
Molybdenum is a transition metal with a high chemical versatility
Activation of inactive-DgAOR assessed by kinetic studies In vivo, DgAOR is expressed and performs its task under anaerobic conditions
Inactive-DgAOR was purified from two batches showing undetectable and very low specific activities (80% inactive)
Summary
Molybdenum is a transition metal with a high chemical versatility. It is the most abundant transition metal in seawater and an essential constituent of a wide variety of biological systems. The high chemical flexibility of molybdenum defines its role in enzymatic systems, where it participates catalyzing both oxygen insertion and abstraction in distinct reactions involved in the carbon, nitrogen, and sulfur metabolism [3,4]. Mo-containing enzymes can be split in two main groups. In the first group the active site comprises a multinuclear heterometallic cluster called FeMoCo which is present in bacterial nitrogenases. The second group comprises enzymes with a mononuclear active site of Mo, which includes the closely related W-containing enzymes [1,2].
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