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PDBsum entry 1yeh
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protein metals Protein-protein interface(s) links
Catalytic antibody PDB id
1yeh

 

 

 

 

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Contents
Protein chains
219 a.a.
222 a.a. *
Metals
_ZN ×7
Waters ×130
* Residue conservation analysis
PDB id:
1yeh
Name: Catalytic antibody
Title: Structure of igg2a fab fragment
Structure: Fab fragment. Chain: l. Other_details: ig gamma-2a chain c region (d2.3). Fab fragment. Chain: h. Other_details: ig gamma-2a chain c region (d2.3)
Source: Fragment: fab. Mus musculus. House mouse. Organism_taxid: 10090. Organism_taxid: 10090
Biol. unit: Tetramer (from PQS)
Resolution:
2.55Å     R-factor:   0.181     R-free:   0.231
Authors: B.Gigant,M.Knossow
Key ref:
B.Gigant et al. (1997). X-ray structures of a hydrolytic antibody and of complexes elucidate catalytic pathway from substrate binding and transition state stabilization through water attack and product release. Proc Natl Acad Sci U S A, 94, 7857-7861. PubMed id: 9223277 DOI: 10.1073/pnas.94.15.7857
Date:
29-May-97     Release date:   03-Dec-97    
PROCHECK
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 Headers
 References

Protein chain
No UniProt id for this chain
Struc: 219 a.a.
Protein chain
Pfam   ArchSchema ?
P01863  (GCAA_MOUSE) -  Ig gamma-2A chain C region, A allele from Mus musculus
Seq:
Struc: 		330 a.a.
222 a.a.
Key:    PfamA domain  Secondary structure  CATH domain

 

 
DOI no: 10.1073/pnas.94.15.7857 Proc Natl Acad Sci U S A 94:7857-7861 (1997)
PubMed id: 9223277  
 
 
X-ray structures of a hydrolytic antibody and of complexes elucidate catalytic pathway from substrate binding and transition state stabilization through water attack and product release.
B.Gigant, J.B.Charbonnier, Z.Eshhar, B.S.Green, M.Knossow.
 
  ABSTRACT  
 
The x-ray structures of the unliganded esterase-like catalytic antibody D2.3 and its complexes with a substrate analogue and with one of the reaction products are analyzed. Together with the structure of the phosphonate transition state analogue hapten complex, these crystal structures provide a complete description of the reaction pathway. At alkaline pH, D2.3 acts by preferential stabilization of the negatively charged oxyanion intermediate of the reaction that results from hydroxide attack on the substrate. A tyrosine residue plays a crucial role in catalysis: it activates the ester substrate and, together with an asparagine, it stabilizes the oxyanion intermediate. A canal allows facile diffusion of water molecules to the reaction center that is deeply buried in the structure. Residues bordering this canal provide targets for mutagenesis to introduce a general base in the vicinity of the reaction center.
 
  Selected figure(s)  
 
Figure 1.
Fig. 1. Chemical reaction catalyzed by D2.3 and structures of the compounds used in this study. Ester 1 is a substrate hydrolyzed^ by D2.3. Crystal structures examined are those of complexes of^ D2.3 with p-nitrobenzyl alcohol 2 (one of the products of the hydrolysis of 1), p-nitrobenzyl phosphonate 3^ (the TSA hapten used to elicit D2.3), and p-nitrobenzyl amide^ 4, a stable analogue of the substrate ester 1. 		Figure 2.
Fig. 2. Schematic views of D2.3 Fab residues that interact with the ligands examined. Residue numbering is according to ref. 24. In A-C, the ligands are in blue, the C[ ]trace of the Fab is in green, and water molecules are in red. Hydrogen bonds are shown as dotted lines. (A) Complex of D2.3 with amide 4, a stable^ SA. (B) Complex of D2.3 with TSA 3. (C) Complex of D2.3^ with the reaction product 2, p-nitrobenzyl alcohol. Electron density corresponding to an acetate molecule was located in the^ combing site. The acetate is in yellow; the oxygens and the methyl of the acetate were distinguished on the basis of the hydrogen bonds established. A-C were drawn with MOLSCRIPT (25). (D) View of the canal (D2.3-4 structure) that allows water diffusion to the carbon atom of the carbonyl of 4 analogous to the^ reaction center in the complex of D2.3 with 1. The surface^ accessible to the exterior of a water molecule represented by a 1.4-Å radius sphere is cut to show the canal; its face toward^ the complexed Fab atoms is in blue, and the one facing the exterior is in white. Only the residues that border the canal are represented. Ligand 4 is in green; the water molecule (magenta) closest to the analogue of the reaction center is within hydrogen bonding distance and angle to Arg-H50 (hydrogen bond not shown). Nitrogen N 1 of His-H35 makes a hydrogen bond to Trp-H47 (not shown) that is conserved in antibodies; therefore, the N 2 nitrogen of His-H35^ (which is part of the canal's wall) is protonated, and His-H35^ most likely does not function as a general base in the hydrolysis catalyzed by D2.3. D was rendered in the AVS environment (26).
 

Literature references that cite this PDB file's key reference

  PubMed id Reference
21190057 J.S.Fraser, and C.J.Jackson (2011).
Mining electron density for functionally relevant protein polysterism in crystal structures.
  Cell Mol Life Sci, 68, 1829-1841.  
19357082 M.Kotaka, R.Kong, I.Qureshi, Q.S.Ho, H.Sun, C.W.Liew, L.P.Goh, P.Cheung, Y.Mu, J.Lescar, and Z.X.Liang (2009).
Structure and catalytic mechanism of the thioesterase CalE7 in enediyne biosynthesis.
  J Biol Chem, 284, 15739-15749.
PDB code: 2w3x
17524985 F.Wang, R.Langley, G.Gulten, L.Wang, and J.C.Sacchettini (2007).
Identification of a type III thioesterase reveals the function of an operon crucial for Mtb virulence.
  Chem Biol, 14, 543-551.
PDB code: 2pfc
15670909 L.Zheng, R.Manetsch, W.D.Woggon, U.Baumann, and J.L.Reymond (2005).
Mechanistic study of proton transfer and hysteresis in catalytic antibody 16E7 by site-directed mutagenesis and homology modeling.
  Bioorg Med Chem, 13, 1021-1029.  
15240887 F.Eghiaian, J.Grosclaude, S.Lesceu, P.Debey, B.Doublet, E.Tréguer, H.Rezaei, and M.Knossow (2004).
Insight into the PrPC-->PrPSc conversion from the structures of antibody-bound ovine prion scrapie-susceptibility variants.
  Proc Natl Acad Sci U S A, 101, 10254-10259.
PDB codes: 1tpx 1tqb 1tqc
14988504 L.Zheng, U.Baumann, and J.L.Reymond (2004).
Molecular mechanism of enantioselective proton transfer to carbon in catalytic antibody 14D9.
  Proc Natl Acad Sci U S A, 101, 3387-3392.
PDB codes: 1uwe 1uwg
11913392 D.J.Tantillo, and K.N.Houk (2002).
Transition state docking: a probe for noncovalent catalysis in biological systems. Application to antibody-catalyzed ester hydrolysis.
  J Comput Chem, 23, 84-95.  
11410373 D.J.Tantillo, and K.N.Houk (2001).
Canonical binding arrays as molecular recognition elements in the immune system: tetrahedral anions and the ester hydrolysis transition state.
  Chem Biol, 8, 535-545.  
11575776 T.Tsumuraya, N.Takazawa, A.Tsunakawa, R.Fleck, and S.Masamune (2001).
Catalytic antibodies induced by a zwitterionic hapten.
  Chemistry, 7, 3748-3755.  
10966475 D.Hilvert (2000).
Critical analysis of antibody catalysis.
  Annu Rev Biochem, 69, 751-793.  
The most recent references are shown first. Citation data come partly from CiteXplore and partly from an automated harvesting procedure. Note that this is likely to be only a partial list as not all journals are covered by either method. However, we are continually building up the citation data so more and more references will be included with time. Where a reference describes a PDB structure, the PDB code is shown on the right.

 

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