Catalytic Mechanism of Retaining α-Galactosidase Belonging to Glycoside Hydrolase Family 97

Glycoside hydrolase family 97 (GH 97) is a unique glycoside family that contains inverting and retaining glycosidases. Of these, BtGH97a (SusB) and BtGH97b (UniProtKB/TrEMBL entry Q8A6L0), derived from Bacteroides thetaiotaomicron, have been characterized as an inverting α-glucoside hydrolase and a...

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Bibliographic Details
Published in:Journal of molecular biology 2009-10, Vol.392 (5), p.1232-1241
Main Authors: Okuyama, Masayuki, Kitamura, Momoyo, Hondoh, Hironori, Kang, Min-Sun, Mori, Haruhide, Kimura, Atsuo, Tanaka, Isao, Yao, Min
Format: Article
Language:English
Subjects:
alpha-Galactosidase - chemistry
alpha-Galactosidase - genetics
alpha-Galactosidase - metabolism
Amino Acid Sequence
arrangement of catalytic residues
Bacteroides - enzymology
Biocatalysis
Catalytic Domain
catalytic mechanism
Conserved Sequence
Crystallography, X-Ray
glycoside hydrolase family 97
Glycoside Hydrolases - chemistry
Glycoside Hydrolases - genetics
Glycoside Hydrolases - metabolism
Models, Molecular
Molecular Sequence Data
Mutagenesis, Site-Directed
Protein Structure, Tertiary
retaining α-galactosidase
three-dimensional structure
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Summary:Glycoside hydrolase family 97 (GH 97) is a unique glycoside family that contains inverting and retaining glycosidases. Of these, BtGH97a (SusB) and BtGH97b (UniProtKB/TrEMBL entry Q8A6L0), derived from Bacteroides thetaiotaomicron, have been characterized as an inverting α-glucoside hydrolase and a retaining α-galactosidase, respectively. Previous studies on the three-dimensional structures of BtGH97a and site-directed mutagenesis indicated that Glu532 acts as an acid catalyst and that Glu439 and Glu508 function as the catalytic base in the inverting mechanism. However, BtGH97b lacks base catalysts but possesses a putative catalytic nucleophilic residue, Asp415. Here, we report that Asp415 in BtGH97b is the nucleophilic catalyst based on the results of crystal structure analysis and site-directed mutagenesis study. Structural comparison between BtGH97b and BtGH97a indicated that OD1 of Asp415 in BtGH97b is located at a position spatially identical with the catalytic water molecule of BtGH97a, which attacks on the anomeric carbon from the β-face (i.e., Asp415 is poised for nucleophilic attack on the anomeric carbon). Site-directed mutagenesis of Asp415 leads to inactivation of the enzyme, and the activity is rescued by an external nucleophilic azide ion. That is, Asp415 functions as a nucleophilic catalyst. The multiple amino acid sequence alignment of GH 97 members indicated that almost half of the GH 97 enzymes possess base catalyst residues at the end of β-strands 3 and 5, while the other half of the family show a conserved nucleophilic residue at the end of β-strand 4. The different positions of functional groups on the β-face of the substrate, which seem to be due to “hopping of the functional group” during evolution, have led to divergence of catalytic mechanism within the same family.
ISSN:0022-2836
1089-8638
DOI:10.1016/j.jmb.2009.07.068