Abstract

N-Bromoacetylethanolamine phosphate rapidly and irreversibly inactivates glucosephosphate isomerase in a pseudo first-order fashion. Ratesaturation effects are observed with a minimum half-life of 4.5 minutes and a half-maximal rate of inactivation at 0.056 mM. Substrates, as well as competitive inhibitors, protect the isomerase from inactivation. Using 14C-labeled N-bromoacetylethanolamine phosphate, the incorporation of approximately one equivalent of inactivator per subunit of isomerase is indicated. After acid hydrolysis, the only modification appears to be the formation of carboxymethyl histidine. These studies indicate that the substrate analogue N-bromoacetylethanolamine phosphate is a specific affinity label that can be used to probe the active site of glucosephosphate isomerase.

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