PDBsum entry: 2cqt

Transferase

PDB-id: 2cqt

Biological unit* = asymmetric unit,
as shown
(*as deduced by PQS)

Contents

Description

Header details

Header records

References

PROCHECK

Protein chains

822 a.a. *

Ligands

BGC ×2

PO4 ×2

GOL ×2

Waters ×931

* Residue conservation analysis

Tools

Clefts Calculation

PDB id:

2cqt

Name:

Transferase

Title:

Crystal structure of cellvibrio gilvus cellobiose phosphorylase crystallized from sodium/potassium phosphate

Structure:

Cellobiose phosphorylase. Chain: a, b. Engineered: yes

Source:

Cellvibrio gilvus. Organism_taxid: 11. Expressed in: escherichia coli bl21(de3). Expression_system_taxid: 469008.

Biological unit:

Dimer (from PQS)

UniProt:

Chains A, B: O66264 (O66264_9GAMM)

Seq:

Struc:

Seq:

Struc:

Seq:

Struc:

Seq:

822 a.a.

Struc:

822 a.a.

Key:

PfamA domain

Secondary structure

Resolution:

2.10Å

R-factor:

0.180

R-free:

0.220

Authors:

M.Hidaka,M.Kitaoka,K.Hayashi,T.Wakagi,H.Shoun,S.Fushinobu

Key ref:

M.Hidaka et al. (2006). Structural dissection of the reaction mechanism of cellobiose phosphorylase.. Biochem J, 398, 37-43. [PubMed id: 16646954] [DOI: 10.1042/BJ20060274]

Date:

20-May-05

Release date:

16-May-06

Related entries:

2cqs
the same protein crystallized from ammonium sulfate

Quick_links

Procheck

Clefts

Surface

Key reference

DOI no: 10.1042/BJ20060274

Biochem J 398:37-43 (2006)

PubMed id: 16646954

Structural dissection of the reaction mechanism of cellobiose phosphorylase.

M.Hidaka, M.Kitaoka, K.Hayashi, T.Wakagi, H.Shoun, S.Fushinobu.

ABSTRACT

Cellobiose phosphorylase, a member of the glycoside hydrolase family 94, catalyses the reversible phosphorolysis of cellobiose into alpha-D-glucose 1-phosphate and D-glucose with inversion of the anomeric configuration. The substrate specificity and reaction mechanism of cellobiose phosphorylase from Cellvibrio gilvus have been investigated in detail. We have determined the crystal structure of the glucose-sulphate and glucose-phosphate complexes of this enzyme at a maximal resolution of 2.0 A (1 A=0.1 nm). The phosphate ion is strongly held through several hydrogen bonds, and the configuration appears to be suitable for direct nucleophilic attack to an anomeric centre. Structural features around the sugar-donor and sugar-acceptor sites were consistent with the results of extensive kinetic studies. When we compared this structure with that of homologous chitobiose phosphorylase, we identified key residues for substrate discrimination between glucose and N-acetylglucosamine in both the sugar-donor and sugar-acceptor sites. We found that the active site pocket of cellobiose phosphorylase was covered by an additional loop, indicating that some conformational change is required upon substrate binding. Information on the three-dimensional structure of cellobiose phosphorylase will facilitate engineering of this enzyme, the application of which to practical oligosaccharide synthesis has already been established.