The Active Site Topology of Aspergillus nigerEndopolygalacturonase II as Studied by Site-directed Mutagenesis

Strictly conserved charged residues among polygalacturonases (Asp-180, Asp-201, Asp-202, His-223, Arg-256, and Lys-258) were subjected to site-directed mutagenesis in Aspergillus niger endopolygalacturonase II. Specific activity, product progression, and kinetic parameters ( K m and V max ) were det...

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Published in:The Journal of biological chemistry 2000-01, Vol.275 (1), p.691-696
Main Authors: Armand, Sylvie, Wagemaker, Matthé J.M., Sánchez-Torres, Paloma, Kester, Harry C.M., van Santen, Yovka, Dijkstra, Bauke W., Visser, Jaap, Benen, Jacques A.E.
Format: Article
Language:English
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Summary:Strictly conserved charged residues among polygalacturonases (Asp-180, Asp-201, Asp-202, His-223, Arg-256, and Lys-258) were subjected to site-directed mutagenesis in Aspergillus niger endopolygalacturonase II. Specific activity, product progression, and kinetic parameters ( K m and V max ) were determined on polygalacturonic acid for the purified mutated enzymes, and bond cleavage frequencies on oligogalacturonates were calculated. Depending on their specific activity, the mutated endopolygalacturonases II were grouped into three classes. The mutant enzymes displayed bond cleavage frequencies on penta- and/or hexagalacturonate different from the wild type endopolygalacturonase II. Based on the biochemical characterization of endopolygalacturonase II mutants together with the three-dimensional structure of the wild type enzyme, we suggest that the mutated residues are involved in either primarily substrate binding (Arg-256 and Lys-258) or maintaining the proper ionization state of a catalytic residue (His-223). The individual roles of Asp-180, Asp-201, and Asp-202 in catalysis are discussed. The active site topology is different from the one commonly found in inverting glycosyl hydrolases.
ISSN:0021-9258
1083-351X
DOI:10.1074/jbc.275.1.691