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PDBsum entry 4lxx
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protein ligands metals Protein-protein interface(s) links
Transferase PDB id
4lxx

 

 

 

 

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Contents
Protein chains
273 a.a.
Ligands
FON ×2
MPO ×4
FNF ×2
EDO ×4
Metals
_CL
Waters ×764
PDB id:
4lxx
Name: Transferase
Title: Crystal structure wlard, a sugar 3n-formyl transferase in the presence of dtdp-fuc3nfo and 5-n-formyl-thf
Structure: Wlard, a sugar 3n-formyl transferase. Chain: a, b. Engineered: yes
Source: Campylobacter jejuni subsp. Jejuni. Organism_taxid: 407148. Strain: 81116. Gene: c8j_1081. Expressed in: escherichia coli. Expression_system_taxid: 562.
Resolution:
1.45Å     R-factor:   0.183     R-free:   0.212
Authors: J.B.Thoden,M.-F.Goneau,M.Gilbert,H.M.Holden
Key ref: J.B.Thoden et al. (2013). Structure of a sugar N-formyltransferase from Campylobacter jejuni. Biochemistry, 52, 6114-6126. PubMed id: 23898784 DOI: 10.1021/bi4009006
Date:
30-Jul-13     Release date:   14-Aug-13    
PROCHECK
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 Headers
 References

Protein chains
A8FMJ3  (A8FMJ3_CAMJ8) - 
Key:    Secondary structure

 

 
DOI no: 10.1021/bi4009006 Biochemistry 52:6114-6126 (2013)
PubMed id: 23898784  
 
 
Structure of a sugar N-formyltransferase from Campylobacter jejuni.
J.B.Thoden, M.F.Goneau, M.Gilbert, H.M.Holden.
 
  ABSTRACT  
 
The O-antigens, which are components of the outer membranes of Gram-negative bacteria, are responsible for the wide species variations seen in nature and are thought to play a role in bacterial virulence. They often contain unusual dideoxysugars such as 3,6-dideoxy-3-formamido-d-glucose (Qui3NFo). Here, we describe a structural and functional investigation of the protein C8J_1081 from Campylobacter jejuni 81116, which is involved in the biosynthesis of Qui3NFo. Specifically, the enzyme, hereafter referred to as WlaRD, catalyzes the N-formylation of dTDP-3,6-dideoxy-3-amino-d-glucose (dTDP-Qui3N) using N(10)-formyltetrahydrofolate as the carbon source. For this investigation, seven X-ray structures of WlaRD, in complexes with various dTDP-linked sugars and cofactors, were determined to resolutions of 1.9 Å or better. One of the models, with bound N(10)-formyltetrahydrofolate and dTDP, represents the first glimpse of an N-formyltransferase with its natural cofactor. Another model contains the reaction products, tetrahydrofolate and dTDP-Qui3NFo. In combination, the structures provide snapshots of the WlaRD active site before and after catalysis. On the basis of these structures, three amino acid residues were targeted for study: Asn 94, His 96, and Asp 132. Mutations of any of these residues resulted in a complete loss of enzymatic activity. Given the position of His 96 in the active site, it can be postulated that it functions as the active site base to remove a proton from the sugar amino group as it attacks the carbonyl carbon of the N-10 formyl group of the cofactor. Enzyme assays demonstrate that WlaRD is also capable of utilizing dTDP-3,6-dideoxy-3-amino-d-galactose (dTDP-Fuc3N) as a substrate, albeit at a much reduced catalytic efficiency.
 

 

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