Structural basis of exo-β-mannanase activity in the GH2 family

Mariane Noronha Domingues; Flavio Henrique Moreira Souza; Plínio Salmazo Vieira; Mariana Abrahão Bueno de Morais; Letícia Maria Zanphorlin; Camila Ramos Dos Santos; Renan Augusto Siqueira Pirolla; Rodrigo Vargas Honorato; Paulo Sergio Lopes de Oliveira; Fabio Cesar Gozzo; Mário Tyago Murakami

doi:10.1074/jbc.RA118.002374

Structural basis of exo-β-mannanase activity in the GH2 family

J Biol Chem. 2018 Aug 31;293(35):13636-13649. doi: 10.1074/jbc.RA118.002374. Epub 2018 Jul 11.

Affiliations

¹ From the Brazilian Bioethanol Science and Technology Laboratory and.
² Brazilian Biosciences National Laboratory, Brazilian Center for Research in Energy and Materials, Campinas, São Paulo 13083-970, Brazil and.
³ the Dalton Mass Spectrometry Laboratory, University of Campinas, Campinas, São Paulo 13083-970, Brazil.
⁴ From the Brazilian Bioethanol Science and Technology Laboratory and mario.murakami@ctbe.cnpem.br.

Abstract

The classical microbial strategy for depolymerization of β-mannan polysaccharides involves the synergistic action of at least two enzymes, endo-1,4-β-mannanases and β-mannosidases. In this work, we describe the first exo-β-mannanase from the GH2 family, isolated from Xanthomonas axonopodis pv. citri (XacMan2A), which can efficiently hydrolyze both manno-oligosaccharides and β-mannan into mannose. It represents a valuable process simplification in the microbial carbon uptake that could be of potential industrial interest. Biochemical assays revealed a progressive increase in the hydrolysis rates from mannobiose to mannohexaose, which distinguishes XacMan2A from the known GH2 β-mannosidases. Crystallographic analysis indicates that the active-site topology of XacMan2A underwent profound structural changes at the positive-subsite region, by the removal of the physical barrier canonically observed in GH2 β-mannosidases, generating a more open and accessible active site with additional productive positive subsites. Besides that, XacMan2A contains two residue substitutions in relation to typical GH2 β-mannosidases, Gly⁴³⁹ and Gly⁵⁵⁶, which alter the active site volume and are essential to its mode of action. Interestingly, the only other mechanistically characterized mannose-releasing exo-β-mannanase so far is from the GH5 family, and its mode of action was attributed to the emergence of a blocking loop at the negative-subsite region of a cleft-like active site, whereas in XacMan2A, the same activity can be explained by the removal of steric barriers at the positive-subsite region in an originally pocket-like active site. Therefore, the GH2 exo-β-mannanase represents a distinct molecular route to this rare activity, expanding our knowledge about functional convergence mechanisms in carbohydrate-active enzymes.

Keywords: GH2 family; Xanthomonas axonopodis pv. citri; enzyme; enzyme catalysis; exo-β-mannanase; glycoside hydrolase; molecular mechanism; protein conformation; protein structure; site-directed mutagenesis.

Publication types

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

MeSH terms

Amino Acid Sequence
Bacterial Proteins / chemistry
Bacterial Proteins / metabolism*
Catalytic Domain
Crystallography, X-Ray
Hydrolysis
Kinetics
Mannans / metabolism
Mannose / metabolism
Models, Molecular
Protein Conformation
Scattering, Small Angle
Sequence Alignment
Substrate Specificity
X-Ray Diffraction
Xanthomonas / chemistry
Xanthomonas / enzymology
Xanthomonas / metabolism*
beta-Mannosidase / chemistry
beta-Mannosidase / metabolism*

Substances

Bacterial Proteins
Mannans
mannobiose
beta-Mannosidase
Mannose

Associated data

PDB/6BYC
PDB/6BYE
PDB/6BYG
PDB/6BYI
PDB/2JE8
PDB/4CVU
PDB/2VX5
PDB/5JU9
PDB/1UUQ
PDB/1WU4
PDB/4PMV
PDB/4KCB