1u0a
From Proteopedia
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Crystal structure of the engineered beta-1,3-1,4-endoglucanase H(A16-M) in complex with beta-glucan tetrasaccharide
Overview
Depolymerization of polysaccharides is catalyzed by highly specific, enzymes that promote hydrolysis of the scissile glycosidic bond by an, activated water molecule. 1,3-1,4-beta-Glucanases selectively cleave, beta-1,4 glycosidic bonds in 3-O-substituted glucopyranosyl units within, polysaccharides with mixed linkage. The reaction follows a, double-displacement mechanism by which the configuration of the anomeric, C(1)-atom of the glucosyl unit in subsite -I is retained. Here we report, the high-resolution crystal structure of the hybrid 1,3-1,4-beta-glucanase, H(A16-M)(E105Q/E109Q) in complex with a beta-glucan tetrasaccharide. The, structure shows four beta-d-glucosyl moieties bound to the, substrate-binding cleft covering subsites -IV to -I, thus corresponding to, the reaction product. The ten active-site residues Asn26, Glu63, Arg65, Phe92, Tyr94, Glu105, Asp107, Glu109, Asn182 and Trp184 form a network of, hydrogen bonds and hydrophobic stacking interactions with the substrate., These residues were previously identified by mutational analysis as, significant for stabilization of the enzyme-carbohydrate complex, with, Glu105 and Glu109 being the catalytic residues. Compared to the Michaelis, complex model, the tetrasaccharide moiety is slightly shifted toward that, part of the cleft binding the non-reducing end of the substrate, but shows, previously unanticipated strong stacking interactions with Phe92 in, subsite -I. A number of specific hydrogen-bond contacts between the enzyme, and the equatorial O(2), O(3) and O(6) hydroxyl groups of the glucosyl, residues in subsites -I, -II and -III are the structural basis for the, observed substrate specificity of 1,3-1,4-beta-glucanases. Kinetic, analysis of enzyme variants with the all beta-1,3 linked polysaccharide, laminarin identified key residues mediating substrate specificity in good, agreement with the structural data. The comparison with structures of the, apo-enzyme H(A16-M) and a covalent enzyme-inhibitor (E.I) complex, together with kinetic and mutagenesis data, yields new insights into the, structural requirements for substrate binding and catalysis. A detailed, view of enzyme-carbohydrate interactions is presented and mechanistic, implications are discussed.
About this Structure
1U0A is a Single protein structure of sequence from Paenibacillus macerans with CA and ZN as ligands. Active as Licheninase, with EC number 3.2.1.73 Full crystallographic information is available from OCA.
Reference
Structural basis for the substrate specificity of a Bacillus 1,3-1,4-beta-glucanase., Gaiser OJ, Piotukh K, Ponnuswamy MN, Planas A, Borriss R, Heinemann U, J Mol Biol. 2006 Apr 7;357(4):1211-25. Epub 2006 Jan 25. PMID:16483609
Page seeded by OCA on Wed Nov 21 03:44:32 2007
