Andrew F. Bury scite author profile

Two main arylamidase activities were separated from a particle-free supernatant of rat heart by chromatography on DEAE-Sephadex. Although both enzymes hydrolysed L-leucine 4-nitroanilide, only peak-II enzyme hydrolysed L-lysine 4-nitroanilide. A third minor peak (Ia) contained an enzyme that was active mainly on the L-lysine 4-nitroanilide. The mol.wts. of the enzymes in peaks I and II were approx. 257000 and 105000 respectively. The pH optimum was approx. pH7.0 for peak-I enzyme and 7.0-8.0 for peak-II enzyme. Both enzymes were inhibited by addition of puromycin, p-hydroxymercuribenzoate, o-phenanthroline and bivalent metal ions. Addition of dithiothreitol resulted in stimulation of both activities. Dialysis against o-phenanthroline resulted in inhibition of peak-I and -II enzymes, but after dialysis against EDTA only peak-II enzyme was inhibited.

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Plasma Arginine Esterase in Cystic Fibrosis: Kinetics of Activation, Identification as Plasma Kallikrein, Reaction with μ2-Macroglobulin and Comparison with Levels in Normal Plasma

Bury

Barrett

1982

Pediatr Res

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Andrew F. Bury

Analysis of protein and peptide mixtures

Hydrolysis of diepptide 2-naphthylamides by human muscle enzymes

Arylamidases in Human Muscle

Separation and properties of two arylamidases from rat cardiac-muscle extracts

Plasma Arginine Esterase in Cystic Fibrosis: Kinetics of Activation, Identification as Plasma Kallikrein, Reaction with μ2-Macroglobulin and Comparison with Levels in Normal Plasma

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