Halide-stabilizing residues of haloalkane dehalogenases studied by quantum mechanic calculations and site-directed mutagenesis
Language English Country United States Media print
Document type Journal Article, Research Support, Non-U.S. Gov't, Validation Study
PubMed
12450392
DOI
10.1021/bi026427v
PII: bi026427v
Knihovny.cz E-resources
- MeSH
- Amino Acids chemistry genetics MeSH
- Anions chemistry MeSH
- Asparagine genetics MeSH
- Models, Chemical MeSH
- Phenylalanine genetics MeSH
- Halogens chemistry MeSH
- Histidine genetics MeSH
- Hydrolases chemistry genetics MeSH
- Isoleucine genetics MeSH
- Quantum Theory * MeSH
- Glutamic Acid genetics MeSH
- Leucine genetics MeSH
- Mathematical Computing MeSH
- Mutagenesis, Site-Directed * MeSH
- Proline genetics MeSH
- Static Electricity MeSH
- Tryptophan genetics MeSH
- Valine genetics MeSH
- Publication type
- Journal Article MeSH
- Research Support, Non-U.S. Gov't MeSH
- Validation Study MeSH
- Names of Substances
- Amino Acids MeSH
- Anions MeSH
- Asparagine MeSH
- Phenylalanine MeSH
- haloalcohol dehalogenase MeSH Browser
- haloalkane dehalogenase MeSH Browser
- Halogens MeSH
- Histidine MeSH
- Hydrolases MeSH
- Isoleucine MeSH
- Glutamic Acid MeSH
- Leucine MeSH
- Proline MeSH
- Tryptophan MeSH
- Valine MeSH
Haloalkane dehalogenases catalyze cleavage of the carbon-halogen bond in halogenated aliphatic compounds, resulting in the formation of an alcohol, a halide, and a proton as the reaction products. Three structural features of haloalkane dehalogenases are essential for their catalytic performance: (i) a catalytic triad, (ii) an oxyanion hole, and (iii) the halide-stabilizing residues. Halide-stabilizing residues are not structurally conserved among different haloalkane dehalogenases. The level of stabilization of the transition state structure of S(N)2 reaction and halide ion provided by each of the active site residues in the enzymes DhlA, LinB, and DhaA was quantified by quantum mechanic calculations. The residues that significantly stabilize the halide ion were assigned as the primary (essential) or the secondary (less important) halide-stabilizing residues. Site-directed mutagenesis was conducted with LinB enzyme to confirm location of its primary halide-stabilizing residues. Asn38Asp, Asn38Glu, Asn38Phe, Asn38Gln, Trp109Leu, Phe151Leu, Phe151Trp, Phe151Tyr, and Phe169Leu mutants of LinB were constructed, purified, and kinetically characterized. The following active site residues were classified as the primary halide-stabilizing residues: Trp125 and Trp175 of DhlA; Asn38 and Trp109 of LinB; and Asn41 and Trp107 of DhaA. All these residues make a hydrogen bond with the halide ion released from the substrate molecule, and their substitution results in enzymes with significantly modified catalytic properties. The following active site residues were classified as the secondary halide-stabilizing residues: Phe172, Pro223, and Val226 of DhlA; Trp207, Pro208, and Ile211 of LinB; and Phe205, Pro206, and Ile209 of DhaA. The differences in the halide stabilizing residues of three haloalkane dehalogenases are discussed in the light of molecular adaptation of these enzymes to their substrates.
References provided by Crossref.org
Discovery of Novel Haloalkane Dehalogenase Inhibitors
