Involvement of surface cysteines in activity and multimer formation of thimet oligopeptidase

doi:10.1093/protein/gzg073

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Protein Engineering vol. 16 no. 8 pp. 623-628, 2003
© 2003 Oxford University Press

Involvement of surface cysteines in activity and multimer formation of thimet oligopeptidase

J.A. Sigman¹, M.L. Sharky¹, S.T. Walsh¹, A. Pabon², M.J. Glucksman² and A.J. Wolfson¹^,3

¹Department of Chemistry, Wellesley College, Wellesley, MA 02481 and ²FUHS/Chicago Medical School, Midwest Proteome Center and Department of Biochemistry and Molecular Biology, Chicago, IL 60064, USA

³ To whom correspondence should be addressed. e-mail: awolfson{at}wellesley.edu

Thimet oligopeptidase is a metalloenzyme involved in regulatingneuropeptide processing. Three cysteine residues (246, 248,253) are known to be involved in thiol activation of the enzyme.In contrast to the wild-type enzyme, the triple mutant (C246S/C248S/C253S)displays increased activity in the absence of dithiothreitol.Dimers, purportedly formed through cysteines 246, 248 and 253,have been thought to be inactive. However, analysis of the triplemutant by native gel electrophoresis reveals the existence ofdimers and multimers, implying that oligomer formation is mediatedby other cysteines, probably on the surface, and that some ofthese forms are enzymatically active. Isolation and characterizationof iodoacetate-modified monomers and dimers of the triple mutantrevealed that, indeed, certain dimeric forms of the enzyme arestill fully active, whereas others show reduced activity. Cysteineresidues potentially involved in dimerization were identifiedby modeling of thimet oliogopeptidase to its homolog, neurolysin.Five mutants were constructed; all contained the triple mutationC246S/C248S/C253S and additional substitutions. Substitutionsat C46 or C682 and C687 prevented multimer formation and inhibiteddimer formation. The C46S mutant had enzymatic activity comparableto the parent triple mutant, whereas that of C682S/C687S wasreduced. Thus, the location of intermolecular disulfide bonds,rather than their existence per se, is relevant to activity.Dimerization close to the N-terminus is detrimental to activity,whereas dimerization near the C-terminus has little effect.Altering disulfide bond formation is a potential regulatoryfactor in the cell owing to the varying oxidation states insubcellular compartments and the different compartmental locationsand functions of the enzyme.

Received March 1, 2003; revised June 17, 2003; accepted June 23, 2003.

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Involvement of surface cysteines in activity and multimer formation of thimet oligopeptidase