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Structure-Based Demystification of Radical Catalysis by a Coenzyme B Dependent Enzyme-Crystallographic Study of Glutamate Mutase with Cofactor Homologues. | LitMetric

Catalysis by radical enzymes dependent on coenzyme B (AdoCbl) relies on the reactive primary 5'-deoxy-5'adenosyl radical, which originates from reversible Co-C bond homolysis of AdoCbl. This bond homolysis is accelerated roughly 10-fold upon binding the enzyme substrate. The structural basis for this activation is still strikingly enigmatic. As revealed here, a displaced firm adenosine binding cavity in substrate-loaded glutamate mutase (GM) causes a structural misfit for intact AdoCbl that is relieved by the homolytic Co-C bond cleavage. Strategically interacting adjacent adenosine- and substrate-binding protein cavities provide a tight caged radical reaction space, controlling the entire radical path. The GM active site is perfectly structured for promoting radical catalysis, including "negative catalysis", a paradigm for AdoCbl-dependent mutases.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10947579PMC
http://dx.doi.org/10.1002/ange.202208295DOI Listing

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