5cpa Citations

Refined crystal structure of carboxypeptidase A at 1.54 A resolution.

Rees DC, Lewis M, Lipscomb WN
J Mol Biol 168 367-87 (1983)
Cited: 204 times
EuropePMC logo PMID: 6887246

Abstract

The crystal structure of bovine carboxypeptidase A (Cox) has been refined at 1.54 A resolution using the restrained least-squares algorithm of Hendrickson & Konnert (1981). The crystallographic R factor (formula; see text) for structure factors calculated from the final model is 0.190. Bond lengths and bond angles in the carboxypeptidase A model have root-mean-square deviations from ideal values of 0.025 A and 3.6 degrees, respectively. Four examples of a reverse turn like structure (the "Asx" turn) requiring an aspartic acid or asparagine residue are observed in this structure. The Asx turn has the same number of atoms as a reverse turn, but only one peptide bond, and the hydrogen bond that closes the turn is between the Asx side-chain CO group and a main-chain NH group. The distributions of CO-N and NH-O hydrogen bond angles in the alpha-helices and beta-sheet structures of carboxypeptidase A are centered about 156 degrees. A total of 192 water molecules per molecule of enzyme are included in the final model. Unlike the hydrogen bonding geometry observed in the secondary structure of the enzyme, the CO-O(wat) hydrogen bond angle is distributed about 131 degrees, indicating the role of the lone pair electrons of the carbonyl oxygen in the hydrogen bond interaction. Twenty four solvent molecules are observed buried within the protein. Several of these waters are organized into hydrogen-bonded chains containing up to five waters. The average temperature factor for atoms in carboxypeptidase A is 8 A2, and varies from 5 A2 in the center of the protein, to over 30 A2 at the surface.

Reviews - 5cpa mentioned but not cited (1)

  1. Overview of protein structural and functional folds. Sun PD, Foster CE, Boyington JC. Curr Protoc Protein Sci Chapter 17 Unit 17.1 (2004)

Articles - 5cpa mentioned but not cited (16)



Reviews citing this publication (15)

  1. Hydrogen bonding in globular proteins. Baker EN, Hubbard RE. Prog Biophys Mol Biol 44 97-179 (1984)
  2. The Hofmeister effect and the behaviour of water at interfaces. Collins KD, Washabaugh MW. Q Rev Biophys 18 323-422 (1985)
  3. Fold change in evolution of protein structures. Grishin NV. J Struct Biol 134 167-185 (2001)
  4. Molecular mechanisms for the conversion of zymogens to active proteolytic enzymes. Khan AR, James MN. Protein Sci 7 815-836 (1998)
  5. Zinc enzymes. Coleman JE. Curr Opin Chem Biol 2 222-234 (1998)
  6. Bacterial dehalogenases: biochemistry, genetics, and biotechnological applications. Fetzner S, Lingens F. Microbiol Rev 58 641-685 (1994)
  7. Zinc hydrolases: the mechanisms of zinc-dependent deacetylases. Hernick M, Fierke CA. Arch Biochem Biophys 433 71-84 (2005)
  8. Energised (entatic) states of groups and of secondary structures in proteins and metalloproteins. Williams RJ. Eur J Biochem 234 363-381 (1995)
  9. Standard structures in proteins. Efimov AV. Prog Biophys Mol Biol 60 201-239 (1993)
  10. Structural trees for protein superfamilies. Efimov AV. Proteins 28 241-260 (1997)
  11. Structure and mechanism of metallocarboxypeptidases. Gomis-Rüth FX. Crit Rev Biochem Mol Biol 43 319-345 (2008)
  12. Designing hydrolytic zinc metalloenzymes. Zastrow ML, Pecoraro VL. Biochemistry 53 957-978 (2014)
  13. Engineered metalloregulation in enzymes. Higaki JN, Fletterick RJ, Craik CS. Trends Biochem Sci 17 100-104 (1992)
  14. Advances in metallo-procarboxypeptidases. Emerging details on the inhibition mechanism and on the activation process. Avilés FX, Vendrell J, Guasch A, Coll M, Huber R. Eur J Biochem 211 381-389 (1993)
  15. Zinc-catalyzed sulfur alkyation:insights from protein farnesyltransferase. Hightower KE, Fierke CA. Curr Opin Chem Biol 3 176-181 (1999)

Articles citing this publication (172)



Related citations provided by authors (7)

Quick links