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Review
. 2009 May;276(9):2447-53.
doi: 10.1111/j.1742-4658.2009.06965.x. Epub 2009 Mar 16.

Reaction mechanisms of thiamin diphosphate enzymes: new insights into the role of a conserved glutamate residue

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Free article
Review

Reaction mechanisms of thiamin diphosphate enzymes: new insights into the role of a conserved glutamate residue

Boaz Shaanan et al. FEBS J. 2009 May.
Free article

Abstract

Subsequent to the demonstration in the late 1950s of the catalytic power of the C2 anion/ylid of thiamin diphosphate, further convincing evidence was provided demonstrating that the 4'-aminopyrimidine group plays a vital role in activation of this cofactor. Structural evidence from several crystal structures of thiamin diphosphate-dependent enzymes emphasized the presence of a glutamate residue in hydrogen-bonding distance from N1' as a conserved element in these enzymes. The important role of this conserved glutamate in promoting C2-H ionization and activation of thiamin diphosphate was emphasized by site-directed mutagenesis studies. This role was further elaborated by spectroscopic studies of the 4'-aminopyrimidine-iminopyrimidine tautomerization. The low polarity of the environment of the protein-bound thiazolium is an additional factor in the stabilization of the C2 anion/ylid. The recently determined crystal structure and mutagenesis studies of glyoxylate carboligase, in which the position of the conserved glutamate is occupied by valine, now show that, for the multi-step reaction catalyzed by this enzyme, the advantages of accelerating the ionization of C2-H by re-introducing a carboxylate are outweighed by the apparent overstabilization of intermediates.

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