What drives chorismate mutase to top performance? Insights from a combinedin silicoandin vitrostudy

Author:

Thorbjørnsrud Helen V.,Bressan Luca,Khatanbaatar TamjidmaaORCID,Carrer ManuelORCID,Würth-Roderer KathrinORCID,Cordara GabrieleORCID,Kast PeterORCID,Cascella MicheleORCID,Krengel UteORCID

Abstract

ABSTRACTUnlike typical chorismate mutases, the enzyme fromMycobacterium tuberculosis(MtCM) has only low activity on its own. Remarkably, its catalytic efficiencykcat/Kmcan be boosted more than 100-fold by complex formation with a partner enzyme. Recently, an autonomously fully active MtCM variant was generated using directed evolution, and its structure solved by X-ray crystallography. However, key residues were involved in crystal contacts, challenging the functional interpretation of the structural changes. Here, we address these challenges by microsecond molecular dynamics simulations, followed up by additional kinetic and structural analyses of selected sets of specifically engineered enzyme variants. A comparison of wild-type MtCM with naturally and artificially activated MtCMs revealed the overall dynamic profiles of these enzymes as well as key interactions between the C-terminus and the active site loop. In the artificially evolved variant of this model enzyme, this loop is pre-organized and stabilized by Pro52 and Asp55, two highly conserved residues in typical, highly active chorismate mutases. Asp55 stretches across the active site and helps to appropriately position active site residues Arg18 and Arg46 for catalysis. The role of Asp55 can be taken over by another acidic residue, if introduced at position 88 close to the C-terminus of MtCM, as suggested by MD simulations and confirmed by kinetic investigations of engineered variants.

Publisher

Cold Spring Harbor Laboratory

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