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PDBsum entry 3bgo
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protein ligands metals Protein-protein interface(s) links
Hydrolase PDB id
3bgo

 

 

 

 

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Contents
Protein chains
71 a.a. *
263 a.a. *
Ligands
AZI
Metals
_ZN ×4
Waters ×293
* Residue conservation analysis
PDB id:
3bgo
Name: Hydrolase
Title: Azide complex of engineered subtilisin subt_bacam
Structure: Subtilisin bpn'. Chain: p. Fragment: prodomain. Synonym: subtilisin novo, subtilisin dfe, alkaline protease. Engineered: yes. Mutation: yes. Subtilisin bpn'. Chain: s. Fragment: enzyme domain.
Source: Bacillus amyloliquefaciens. Organism_taxid: 1390. Gene: apr. Expressed in: escherichia coli. Expression_system_taxid: 562. Expression_system_taxid: 562
Resolution:
1.80Å     R-factor:   0.208     R-free:   0.262
Authors: D.T.Gallagher,P.N.Bryan
Key ref: T.Gallagher et al. (2009). Structure of a switchable subtilisin complexed with a substrate and with the activator azide. Biochemistry, 48, 10389-10394. PubMed id: 19761257
Date:
27-Nov-07     Release date:   03-Jun-08    
PROCHECK
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 Headers
 References

Protein chain
Pfam   ArchSchema ?
P00782  (SUBT_BACAM) -  Subtilisin BPN' from Bacillus amyloliquefaciens
Seq:
Struc: 		382 a.a.
71 a.a.*
Protein chain
Pfam   ArchSchema ?
P00782  (SUBT_BACAM) -  Subtilisin BPN' from Bacillus amyloliquefaciens
Seq:
Struc: 		382 a.a.
263 a.a.*
Key:    PfamA domain  Secondary structure  CATH domain
* PDB and UniProt seqs differ at 35 residue positions (black crosses)

 Enzyme reactions 
   Enzyme class: Chains P, S: E.C.3.4.21.62  - subtilisin.
[IntEnz]   [ExPASy]   [KEGG]   [BRENDA]
      Reaction: Hydrolysis of proteins with broad specificity for peptide bonds, and a preference for a large uncharged residue in P1. Hydrolyzes peptide amides.

 

 
Biochemistry 48:10389-10394 (2009)
PubMed id: 19761257  
 
 
Structure of a switchable subtilisin complexed with a substrate and with the activator azide.
T.Gallagher, B.Ruan, M.London, M.A.Bryan, P.N.Bryan.
 
  ABSTRACT  
 
An engineered variant of the protease subtilisin from Bacillus amyloliquefaciens, in which the D32A mutation renders the enzyme's activity dependent on the presence of certain small anions such as fluoride or azide, has been produced. This modified enzyme has applications as an azide or fluoride-triggered expression-purification tool. We report activity measurements showing that the enzyme is activated more than 3000-fold by azide and describe the 1.8 A resolution structure of an inactive form (by replacing the catalytic nucleophile Ser 221 with alanine) of the protease, in complex with azide and with a substrate that spans the active site. Both enzyme and substrate have been engineered to increase their stability and the affinity of their interaction. The substrate is based on a stabilized subtilisin prodomain, extended across the active site by the addition of four residues at its C-terminus. In the crystal structure, the substrate is well-ordered across the active site, and the azide anion is observed bound adjacent to Ala 32. The structures of the substrate complex in three different crystals (anion-free, fluoride-soaked, and azide-soaked) are compared. These structures provide extensive information for understanding subtilisin's substrate binding and catalytic mechanism, and for the development of biotechnology tools based on anion-activated proteolysis. The mechanism of anion-dependent proteolysis appears to be a slight modification of the accepted charge-relay mechanism for serine proteases.
 

 

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