Crystal Structure of Bifunctional Aldos-2-Ulose Dehydratase/Isomerase from Phanerochaete chrysosporium with the Reaction Intermediate Ascopyrone M

Crystal Structure of Bifunctional Aldos-2-Ulose Dehydratase/Isomerase from Phanerochaete chrysosporium with the Reaction Intermediate Ascopyrone M

The enzyme aldos-2-ulose dehydratase/isomerase (AUDH) participates in carbohydrate secondary metabolism, catalyzing the conversion of glucosone and 1,5-d-anhydrofructose to the secondary metabolites cortalcerone and microthecin, respectively. AUDH is a homo-dimeric enzyme with subunits of 900 amino...

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Veröffentlicht in:Journal of molecular biology 2012-04, Vol.417 (4), p.279-293
Hauptverfasser: Claesson, Magnus, Lindqvist, Ylva, Madrid, Susan, Sandalova, Tatyana, Fiskesund, Roland, Yu, Shukun, Schneider, Gunter
Format: Artikel
Sprache:eng
Schlagworte:
active sites
Amino Acid Sequence
amino acids
carbon
catalytic activity
Catalytic Domain
crystal structure
Crystallography, X-Ray
cupin fold
enzyme activity
enzyme mechanism
Fructose - analogs & derivatives
Fructose - chemistry
Hydro-Lyases - chemistry
ions
Ketoses - chemistry
lectins
magnesium
metabolism
metalloenzyme
Molecular Sequence Data
Phanerochaete - enzymology
Phanerochaete chrysosporium
propeller domain
protein structure
Protein Structure, Tertiary
protein subunits
secondary metabolites
zinc
Zinc - chemistry
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Zusammenfassung:The enzyme aldos-2-ulose dehydratase/isomerase (AUDH) participates in carbohydrate secondary metabolism, catalyzing the conversion of glucosone and 1,5-d-anhydrofructose to the secondary metabolites cortalcerone and microthecin, respectively. AUDH is a homo-dimeric enzyme with subunits of 900 amino acids. The subunit consists of a seven-bladed β-propeller domain, two cupin folds and a C-terminal lectin domain. AUDH contains a structural Zn2+ and Mg2+ located in loop regions and two zinc ions at the bottom of two putative active-site clefts in the propeller and the cupin domain, respectively. Catalysis is dependent on these two zinc ions, as their specific removal led to loss of enzymatic activity. The structure of the Zn2+-depleted enzyme is very similar to that of native AUDH, and structural changes upon metal removal as the cause for the catalytic deficiencies can be excluded. The complex with the reaction intermediate ascopyrone M shows binding of this compound at two different sites, with direct coordination to Zn2+ in the propeller domain and as second sphere ligand of the metal ion in the cupin domain. These observations suggest that the two reactions of AUDH might be catalyzed in two different active sites, about 60 Å apart. The dehydration reaction most likely follows an elimination mechanism, where Zn2+ acts as a Lewis acid polarizing the C2 keto group of 1,5-d-anhydrofructose. Abstraction of the proton at the C3 carbon atom and protonation of the leaving group, the C4 hydroxyl moiety, could potentially be catalyzed by the side chain of the suitably positioned residue His155. [Display omitted] ► Bifunctional AUDH participates in carbohydrate metabolism. ► The enzyme subunit consists of a β-propeller, a bicupin and a lectin domain. ► The enzyme contains two catalytic zinc ions and one structural zinc ion. ► The reaction intermediate ascopyrone M binds at two different putative active sites.
ISSN:0022-2836
1089-8638
DOI:10.1016/j.jmb.2012.02.001