Your search keyword '"Andrew S. W. Quon"' showing total 2 results

1. The Catalytic Core of Peptidylglycine .alpha.-Hydroxylating Monooxygenase: Investigation by Site-Directed Mutagenesis, Cu X-ray Absorption Spectroscopy, and Electron Paramagnetic Resonance

Author

Betty A. Eipper, Richard E. Mains, Andrew S. W. Quon, John S. Boswell, and Ninian J. Blackburn

Subjects

Stereochemistry, Molecular Sequence Data, Mutant, Peptidylglycine monooxygenase, Photochemistry, Biochemistry, Catalysis, Cell Line, Mixed Function Oxygenases, Substrate Specificity, Multienzyme Complexes, Animals, Amino Acid Sequence, Binding site, Site-directed mutagenesis, Peptide sequence, chemistry.chemical_classification, Binding Sites, biology, Chemistry, Spectrum Analysis, X-Rays, Electron Spin Resonance Spectroscopy, Active site, Monooxygenase, Rats, Kinetics, Enzyme, Mutagenesis, Site-Directed, biology.protein, Cattle, Oligopeptides, Copper

Abstract

Peptidylglycine alpha-hydroxylating monooxygenase (PHM) is a copper, ascorbate, and molecular oxygen dependent enzyme that plays a key role in the biosynthesis of many peptides. Using site-directed mutagenesis, the catalytic core of PHM was found not to extend beyond Asp359. Shorter PHM proteins were eliminated intracellularly, suggesting that they failed to fold correctly. A set of mutant PHM proteins whose design was based on the structural and mechanistic similarities of PHM and dopamine beta-monooxygenase (D beta M) was characterized. Mutation of Tyr79, the residue equivalent to a p-cresol target in D beta M, to Phe79 altered the kinetic parameters of PHM. Disruption of either His-rich cluster contained within the PHM/D beta M homology domain eliminated activity, while deletion of a third His-rich cluster unique to PHM failed to affect activity; the catalytically inactive mutant PHM proteins still bound to a peptidylglycine substrate affinity resin. EPR and EXAFS studies of oxidized PHM indicate that the active site contains type 2 copper in a tetragonal environment; the copper is coordinated to two to three His and one to two additional O/N ligands, probably solvent, again supporting the structural homology of PHM and D beta M. Mutation of the Met residues common to PHM and D beta M to Ile identified Met314 as critical for catalytic activity.

Published

1995

2. Peptidylglycine alpha-hydroxylating monooxygenase: active site residues, disulfide linkages, and a two-domain model of the catalytic core

Author

Betty A. Eipper, Richard E. Mains, Henry T. Keutmann, Aparna S. Kolhekar, and and Andrew S. W. Quon

Subjects

Models, Molecular, Binding Sites, biology, Edman degradation, Chemistry, Stereochemistry, Active site, Peptidylglycine monooxygenase, Monooxygenase, Sulfides, Biochemistry, Mixed Function Oxygenases, Enzyme Activation, Models, Chemical, Multienzyme Complexes, biology.protein, Animals, Humans, Enzyme kinetics, Binding site, Linker, Cysteine

Abstract

Peptidylglycine alpha-hydroxylating monooxygenase (PHM) is a copper, ascorbate, and molecular oxygen dependent enzyme that catalyzes the first step leading to the C-terminal amidation of glycine-extended peptides. The catalytic core of PHM (PHMcc), refined to residues 42-356 of the PHM protein, was expressed at high levels in CHO (DG44) (dhfr-) cells. PHMcc has 10 cysteine residues involved in 5 disulfide linkages. Endoprotease Lys-C digestion of purified PHMcc under nonreducing conditions cleaved the protein at Lys219, indicating that the protein consists of separable N- and C-terminal domains with internal disulfide linkages, that are connected by an exposed linker region. Disulfide-linked peptides generated by sequential CNBr and pepsin treatment of radiolabeled PHMcc were separated by reverse phase HPLC and identified by Edman degradation. Three disulfide linkages occur in the N-terminal domain (Cys47-Cys186, Cys81-Cys126, and Cys114-Cys131), along with three of the His residues critical to catalytic activity (His107, His108, and His172). Two disulfide linkages (Cys227-Cys334 and Cys293-Cys315) occur in the C-terminal domain, along with the remaining two essential His residues (His242, His244) and Met314, thought to be essential in binding one of the two nonequivalent copper atoms. Substitution of Tyr79 or Tyr318 with Phe increased the Km of PHM for its peptidylglycine substrate without affecting the Vmax. Replacement of Glu313 with Asp increased the Km 8-fold and decreased the kcat 7-fold, again identifying this region of the C-terminal domain as critical to catalytic activity. Taking into account information on the copper ligands in PHM, we propose a two-domain model with a copper site in each domain that allows spatial proximity between previously described copper ligands and residues identified as catalytically important.

Published

1997