Degradation and synthesis of β-glucans by a Magnaporthe oryzae endotransglucosylase, a member of the glycoside hydrolase 7 family

Machiko Takahashi; Koichi Yoshioka; Tomoya Imai; Yuka Miyoshi; Yuki Nakano; Kentaro Yoshida; Tetsuro Yamashita; Yuzo Furuta; Takashi Watanabe; Junji Sugiyama; Takumi Takeda

doi:10.1074/jbc.M112.448902

Degradation and synthesis of β-glucans by a Magnaporthe oryzae endotransglucosylase, a member of the glycoside hydrolase 7 family

J Biol Chem. 2013 May 10;288(19):13821-30. doi: 10.1074/jbc.M112.448902. Epub 2013 Mar 25.

Authors

Machiko Takahashi¹, Koichi Yoshioka, Tomoya Imai, Yuka Miyoshi, Yuki Nakano, Kentaro Yoshida, Tetsuro Yamashita, Yuzo Furuta, Takashi Watanabe, Junji Sugiyama, Takumi Takeda

Affiliation

¹ Iwate Biotechnology Research Center, 22-174-4, Narita Kitakami, Iwate 024-0003, Japan.

Abstract

Background: Plant pathogens secrete enzymes that degrade plant cell walls to enhance infection and nutrient acquisition.

Results: A novel endotransglucosylase catalyzes cleavage and transfer of β-glucans and decreases the physical strength of plant cell walls.

Conclusion: Endotransglucosylation causes depolymerization and polymerization of β-glucans, depending on substrate molecular size.

Significance: Enzymatic degradation of plant cell walls is required for wall loosening, which enhances pathogen invasion. A Magnaporthe oryzae enzyme, which was encoded by the Mocel7B gene, was predicted to act on 1,3-1,4-β-glucan degradation and transglycosylation reaction of cellotriose after partial purification from a culture filtrate of M. oryzae cells, followed by liquid chromatography-tandem mass spectrometry. A recombinant MoCel7B prepared by overexpression in M. oryzae exhibited endo-typical depolymerization of polysaccharides containing β-1,4-linkages, in which 1,3-1,4-β-glucan was the best substrate. When cellooligosaccharides were used as the substrate, the recombinant enzyme generated reaction products with both shorter and longer chain lengths than the substrate. In addition, incorporation of glucose and various oligosaccharides including sulforhodamine-conjugated cellobiose, laminarioligosaccharides, gentiobiose, xylobiose, mannobiose, and xyloglucan nonasaccharide into β-1,4-linked glucans were observed after incubation with the enzyme. These results indicate that the recombinant enzyme acts as an endotransglucosylase (ETG) that cleaves the glycosidic bond of β-1,4-glucan as a donor substrate and transfers the cleaved glucan chain to another molecule functioning as an acceptor substrate. Furthermore, ETG treatment caused greater extension of heat-treated wheat coleoptiles. The result suggests that ETG functions to induce wall loosening by cleaving the 1,3-1,4-β-glucan tethers of plant cell walls. On the other hand, use of cellohexaose as a substrate for ETG resulted in the production of cellulose II with a maximum length (degree of polymerization) of 26 glucose units. Thus, ETG functions to depolymerize and polymerize β-glucans, depending on the size of the acceptor substrate.

Keywords: Cell Wall; Cell Wall-degrading Enzymes; Cellulase; Enzyme Purification; Enzymes; Glycobiology.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Carbohydrate Conformation
Cell Wall / chemistry
Cellulose / biosynthesis
Cloning, Molecular
Cotyledon / chemistry
Cotyledon / cytology
Fungal Proteins / chemistry*
Fungal Proteins / genetics
Fungal Proteins / metabolism
Glycoside Hydrolases / chemistry*
Glycoside Hydrolases / genetics
Glycoside Hydrolases / metabolism
Hydrolysis
Magnaporthe / enzymology*
Oligosaccharides / chemistry
Oryza / microbiology
Plant Leaves / microbiology
Substrate Specificity
Transcription, Genetic
Triticum / chemistry
Triticum / cytology
beta-Glucans / metabolism*

Substances

Fungal Proteins
Oligosaccharides
beta-Glucans
Cellulose
Glycoside Hydrolases