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PDBsum entry 1n4f
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protein ligands metals links
Hydrolase PDB id
1n4f

 

 

 

 

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Contents
Protein chain
129 a.a. *
Ligands
ASR ×3
EDO ×5
Metals
_NA
Waters ×121
* Residue conservation analysis
PDB id:
1n4f
Name: Hydrolase
Title: Para-arsanilate derivative of hen egg-white lysozyme
Structure: LysozymE C. Chain: a. Synonym: 1,4-beta-n-acetylmuramidasE C, allergen gal d 4, gal d iv. Ec: 3.2.1.17
Source: Gallus gallus. Chicken. Organism_taxid: 9031. Other_details: hen egg white
Resolution:
1.78Å     R-factor:   0.164     R-free:   0.213
Authors: P.Retailleau,T.Prange
Key ref:
P.Retailleau and T.Prangé (2003). Phasing power at the K absorption edge of organic arsenic. Acta Crystallogr D Biol Crystallogr, 59, 887-896. PubMed id: 12777806 DOI: 10.1107/S0907444903003512
Date:
31-Oct-02     Release date:   06-May-03    
PROCHECK
Go to PROCHECK summary
 Headers
 References

Protein chain
Pfam   ArchSchema ?
P00698  (LYSC_CHICK) -  Lysozyme C from Gallus gallus
Seq:
Struc: 		147 a.a.
129 a.a.
Key:    PfamA domain  Secondary structure  CATH domain

 Enzyme reactions 
   Enzyme class: E.C.3.2.1.17  - lysozyme.
[IntEnz]   [ExPASy]   [KEGG]   [BRENDA]
      Reaction: Hydrolysis of the 1,4-beta-linkages between N-acetyl-D-glucosamine and N-acetylmuramic acid in peptidoglycan heteropolymers of the prokaryotes cell walls.

 

 
DOI no: 10.1107/S0907444903003512 Acta Crystallogr D Biol Crystallogr 59:887-896 (2003)
PubMed id: 12777806  
 
 
Phasing power at the K absorption edge of organic arsenic.
P.Retailleau, T.Prangé.
 
  ABSTRACT  
 
Single/multiple-wavelength anomalous dispersion (SAD/MAD) experiments were performed on a crystal of an organic arsenic derivative of hen egg-white lysozyme. A para-arsanilate compound used as a crystallizing reagent was incorporated into the ordered solvent region of the lysozyme molecule. Diffraction data were collected to high resolution (</=2.0 A) at three wavelengths around the K edge (1.04 A) of arsenic at beamline BM30A, ESRF synchrotron. Anomalous Patterson maps clearly showed the main arsanilate site to be between three symmetry-related lysozyme molecules, at a location previously occupied by a para-toluenesulfonate anion. MAD phases at 2 A derived using the program SHARP led to an electron-density map of sufficient quality to start manual building of the protein model. Amplitudes from a second crystal measured to a resolution of 1.8 A at the peak wavelength revealed two additional heavy-atom sites, which reinforced the anomalous subset model and therefore dramatically improved the phasing power of the arsenic derivative. The subsequent solvent-flattened map was of such high accuracy that the program ARP/wARP was able to build a nearly complete model automatically. This work emphasizes the great potential of arsenic for de novo structure determination using anomalous dispersion methods.
 
  Selected figure(s)  
 
Figure 2.
Figure 2 Resolution-dependent statistics of the anomalous signal and of quality indicators for two different data sets (blue for crystal 1 and black for crystal 2): | F[anom]|/ ( F[anom]) and I/ (I) on the left y axis are absolute numbers, whereas R[sym] and | F[anom]|/F are measured in percentages on the right y axis. 		Figure 3.
Figure 3 {w = 1/2, 0 [216]<= u [217]<= 1/2, 0 [218]<= v [219]<= 1/2} Harker sections of anomalous difference Patterson maps for (a) crystal 1 and (b) crystal 2. Levels are contoured in 1 [220][sigma] steps starting at 2 [221][sigma] .
 
  The above figures are reprinted by permission from the IUCr: Acta Crystallogr D Biol Crystallogr (2003, 59, 887-896) copyright 2003.  
  Figures were selected by an automated process.  

 

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