Open AccessA Single Point Mutation Alters the Transglycosylation/Hydrolysis Partition, Significantly Enhancing the Synthetic Capability of an endo-Glycoceramidase
Author(s) -
Julien Durand,
Xevi Biarnés,
Laurie Watterlot,
Cyrielle Bonzom,
Vinciane Borsenberger,
Antoni Planas,
Sophie Bozonnet,
Michael O’Donohue,
Régis Fauré
Publication year - 2016
Publication title -
acs catalysis
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 4.898
H-Index - 198
ISSN - 2155-5435
DOI - 10.1021/acscatal.6b02159
Subject(s) - chemistry , hydrolysis , substrate (aquarium) , catalysis , stereoselectivity , mutant , alkyl , stereochemistry , glycoside , biocatalysis , ketone , organic chemistry , biochemistry , reaction mechanism , gene , oceanography , geology
The mutation of D311 to tyrosine in endo-glycoceramidase II from Rhodococcus sp. and the use of a poorly recognized substrate, 2-chloro-4-nitrophenyl beta-cellobioside, have provided appropriate conditions for the efficient synthesis of alkyl beta-cellobioside derivatives. The mutant D311Y was characterized by a lowered KM value for the hydrolysis of 2-chloro-4-nitrophenyl beta-cellobioside and increased transglycosylation when using aliphatic 1,3-diols or alcohols bearing a delta-hydroxy ketone function as acceptors. Closer analysis revealed that the transglycosylation/hydrolysis ratio in reactions catalyzed by the mutant was completely inversed and weak secondary hydrolysis was postponed, thus providing the basis for high transglycosylation yields (between 68 and 93%). Overall, results confirm that the enhancement of transglycosylation in glycoside hydrolases can be achieved by a combination of destabilized transition states and increased recognition for acceptor molecules
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