Publication | Open Access
Combinatorial exploration of the catalytic site of a drug-resistant dihydrofolate reductase: creating alternative functional configurations
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Citations
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References
2004
Year
Bioorganic ChemistryAldo-keto ReductaseMolecular BiologyChemical BiologyRedox BiologyActive Site VariantsAlternative Functional ConfigurationsStructure-function Enzyme KineticsAldehyde DehydrogenaseBiochemistryBiocatalysisDirected EvolutionCatalytic SiteActive SiteActive Site ExplorationNatural SciencesEnzyme CatalysisSynthetic BiologyEnzyme SpecificityProtein EngineeringCombinatorial Exploration
We have applied a global approach to enzyme active site exploration, where multiple mutations were introduced combinatorially at the active site of Type II R67 dihydrofolate reductase (R67 DHFR), creating numerous new active site environments within a constant framework. By this approach, we combinatorially modified all 16 principal amino acids that constitute the active site of this enzyme. This approach is fundamentally different from active site point mutation in that the native active site context is no longer accounted for. Among the 1536 combinatorially mutated active site variants of R67 DHFR we created, we selected and kinetically characterized three variants with highly altered active site compositions. We determined that they are of high fitness, as defined by a complex function consisting jointly of catalytic activity and resistance to trimethoprim. The k(cat) and K(M) values were similar to those for the native enzyme. The favourable Delta(DeltaG) values obtained (ranging from -0.72 to -1.08 kcal/mol) suggest that, despite their complex mutational pattern, no fundamental change in the catalytic mechanism has occurred. We illustrate that combinatorial active site mutagenesis can allow for the creation of compensatory mutations that could not be predicted and thus provides a route for more extensive exploration of functional sequence space than is allowed by point mutation.
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