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Impaired Acid Catalysis by Mutation of a Protein Loop Hinge Residue in a YopH Mutant Revealed by Crystal Structures
- Publication Year :
- 2009
-
Abstract
- Catalysis by the Yersinia protein-tyrosine phosphatase YopH is significantly impaired by the mutation of the conserved Trp354 residue to Phe. Though not a catalytic residue, this Trp is a hinge residue in a conserved flexible loop (the WPD-loop) that must close during catalysis. To learn why this seemingly conservative mutation reduces catalysis by 2 orders of magnitude, we have solved high-resolution crystal structures for the W354F YopH in the absence and in the presence of tungstate and vanadate. Oxyanion binding to the P-loop in W354F is analogous to that observed in the native enzyme. However, the WPD-loop in the presence of oxyanions assumes a half-closed conformation, in contrast to the fully closed state observed in structures of the native enzyme. This observation provides an explanation for the impaired general acid catalysis observed in kinetic experiments with Trp mutants. A 1.4 A structure of the W354F mutant obtained in the presence of vanadate reveals an unusual divanadate species with a cyclic [VO](2) core, which has precedent in small molecules but has not been previously reported in a protein crystal structure.
- Subjects :
- Models, Molecular
Stereochemistry
Protein Conformation
Mutant
Phosphatase
Conservative mutation
Crystallography, X-Ray
Biochemistry
Article
Catalysis
Acid catalysis
Residue (chemistry)
Colloid and Surface Chemistry
Protein structure
Catalytic Domain
Hydrolase
Escherichia coli
Vanadate
Chemistry
General Chemistry
Tungsten Compounds
Recombinant Proteins
Crystallography
Mutation
Protein Tyrosine Phosphatases
Vanadates
Bacterial Outer Membrane Proteins
Subjects
Details
- Language :
- English
- Database :
- OpenAIRE
- Accession number :
- edsair.doi.dedup.....c44b54a64a66f423b3f2e7c77766cbfd