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. 1998 Mar 20;279(5358):1958-61.
doi: 10.1126/science.279.5358.1958.

Redesigning enzyme topology by directed evolution

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Redesigning enzyme topology by directed evolution

G MacBeath et al. Science. .

Abstract

Genetic selection was exploited in combination with structure-based design to transform an intimately entwined, dimeric chorismate mutase into a monomeric, four-helix-bundle protein with near native activity. Successful reengineering depended on choosing a thermostable starting protein, introducing point mutations that preferentially destabilize the wild-type dimer, and using directed evolution to optimize an inserted interhelical turn. Contrary to expectations based on studies of other four-helix-bundle proteins, only a small fraction of possible turn sequences (fewer than 0.05 percent) yielded well-behaved, monomeric, and highly active enzymes. Selection for catalytic function thus provides an efficient yet stringent method for rapidly assessing correctly folded polypeptides and may prove generally useful for protein design.

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Comment in

  • The bare bones of catalysis.
    Stokstad E. Stokstad E. Science. 1998 Mar 20;279(5358):1852. doi: 10.1126/science.279.5358.1852. Science. 1998. PMID: 9537901 No abstract available.

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