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1AEH

SPECIFICITY OF LIGAND BINDING TO A BURIED POLAR CAVITY AT THE ACTIVE SITE OF CYTOCHROME C PEROXIDASE (2-AMINO-4-METHYLTHIAZOLE)

Summary for 1AEH
Entry DOI10.2210/pdb1aeh/pdb
DescriptorCYTOCHROME C PEROXIDASE, PROTOPORPHYRIN IX CONTAINING FE, 2-AMINO-4-METHYLTHIAZOLE, ... (4 entities in total)
Functional Keywordsoxidoreductase, peroxidase, transit peptide
Biological sourceSaccharomyces cerevisiae (baker's yeast)
Cellular locationMitochondrion matrix: P00431
Total number of polymer chains1
Total formula weight34189.90
Authors
Musah, R.A.,Jensen, G.M.,Fitzgerald, M.M.,Mcree, D.E.,Goodin, D.B. (deposition date: 1997-02-24, release date: 1997-09-04, Last modification date: 2024-05-22)
Primary citationMusah, R.A.,Jensen, G.M.,Bunte, S.W.,Rosenfeld, R.J.,Goodin, D.B.
Artificial protein cavities as specific ligand-binding templates: characterization of an engineered heterocyclic cation-binding site that preserves the evolved specificity of the parent protein.
J.Mol.Biol., 315:845-857, 2002
Cited by
PubMed Abstract: Cavity complementation has been observed in many proteins, where an appropriate small molecule binds to a cavity-forming mutant. Here, the binding of compounds to the W191G cavity mutant of cytochrome c peroxidase is characterized by X-ray crystallography and binding thermodynamics. Unlike cavities created by removal of hydrophobic side-chains, the W191G cavity does not bind neutral or hydrophobic compounds, but displays a strong specificity for heterocyclic cations, consistent with the role of the protein to stabilize a tryptophan radical at this site. Ligand dissociation constants for the protonated cationic state ranged from 6 microM for 2-amino-5-methylthiazole to 1 mM for neutral ligands, and binding was associated with a large enthalpy-entropy compensation. X-ray structures show that each of 18 compounds with binding behavior bind specifically within the artificial cavity and not elsewhere in the protein. The compounds make multiple hydrogen bonds to the cavity walls using a subset of the interactions seen between the protein and solvent in the absence of ligand. For all ligands, every atom that is capable of making a hydrogen bond does so with either protein or solvent. The most often seen interaction is to Asp235, and most compounds bind with a specific orientation that is defined by their ability to interact with this residue. Four of the ligands do not have conventional hydrogen bonding atoms, but were nevertheless observed to orient their most polar CH bond towards Asp235. Two of the larger ligands induce disorder in a surface loop between Pro190 and Asn195 that has been identified as a mobile gate to cavity access. Despite the predominance of hydrogen bonding and electrostatic interactions, the small variation in observed binding free energies were not correlated readily with the strength, type or number of hydrogen bonds or with calculated electrostatic energies alone. Thus, as with naturally occurring binding sites, affinities to W191G are likely to be due to a subtle balance of polar, non-polar, and solvation terms. These studies demonstrate how cavity complementation and judicious choice of site can be used to produce a protein template with an unusual ligand-binding specificity.
PubMed: 11812152
DOI: 10.1006/jmbi.2001.5287
PDB entries with the same primary citation
Experimental method
X-RAY DIFFRACTION (2.1 Å)
Structure validation

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