On the unimolecular nature of the enzyme tyrosinase

Mallette, M. Frank

January 1945

Thesis (Ph. D.)--Columbia University, 1945. / "Lithoprinted ... Edwards Brothers, Inc., Ann Arbor, Michigan, 1946." Vita. Bibliography: p. 59-60.

Phenol oxidase.

Biocatalysis of tyrosinase in organic solvent media using phenolic substrate models

Bao, Haihong.

January 1999

The biocatalysis of tyrosinase was investigated in selected organic solvent media, using catechin as substrate. The results showed that the optimal enzymatic activity was obtained at pH 6.2, 6.6, 6.0 and 6.2 in heptane, toluene, dichloromethane and dichloroethane media, respectively. The kinetic studies indicated that the Km values were 5.38, 1.03, 2.52 and 4.03 mM, for the enzymatic reaction in heptane, toluene, dichloromethane and dichloroethane media, respectively, whereas the Vmax values were 12.2 x 10--4, 3.3 x 10--4, 14.7 x 10--4 and 12.0 x 10--4 deltaA mug protein--1 sec--1 , respectively. The results showed that the change in acetone concentration, used as co-solvent for the tyrosinase biocatalysis, from 5 to 30% (v/v) in the heptane medium resulted in a decrease of 4.3 to 96.7% in enzymatic activity. However, the presence of 12.5, 22.0 and 22.0% of acetone in the media of dichloromethane, dichloroethane and toluene resulted in a maximal increase in enzymatic activity of 42.6, 71.8 and 92.1%, respectively. Moreover, the biocatalysis of tyrosinase in dichloromethane and heptane reaction media, using model phenolic substrates was also investigated. The Km values for the tyrosinase biocatalysis in dichloromethane medium, using 4-methyl catechol, catechol and catechin as substrates, were 2.21, 2.36 and 2.52 mM, respectively, whereas the Vmax values were 5.1 x 10--4 , 6.0 x 10--4 and 14.7 x 10 --4 deltaA mug protein--1 sec --1, respectively. In addition, the Km values for tyrosinase biocatalysis in the heptane medium, using p-cresol, catechol and catechin as substrates, were 1.07, 4.32 and 5.38 mM, respectively, whereas the Vmax values were 0.8 x 10--4, 1.0 x 10 --4 and 12.2 x 10--3 deltaA mug protein--1 sec--1, respectively. The characterization of the end products resulting from the tyrosinase biocatalysis, using selected substrates, was carried out by spectrophotometeric scanning, differential scanning calorimetry and pyrolysis/gas chromatography coupled to

Phenol oxidase.

Polyphenol oxidase.

Calibration of phenol oxidase measurement in acidic wetland environments

Chanton, Patrick

27 August 2014

Phenol oxidases mediate the degradation of recalcitrant compounds, polyphenolics, in wetland soils and are considered to play a key role in the microbial carbon cycle of peatlands which predominate in boreal biomes. In order to validate a method for quantification of oxidative enzyme activity in acidic wetland environments, the relationship between pH and substrate oxidation was studied using the standard enzyme tyrosinase and in soils collected from six freshwater wetlands including three marshes in north Florida and peatlands of northern Minnesota. Phenol oxidase (PO) activity was quantified with two commonly used assay substrates, ABTS (2,2'-azino-bis(3-ethylobenzthiazoline-6-sulfonic acid) and L-DOPA (L-3,4-dihydroxyphenylalanine), across a pH range of 4 to 7 which matched the in situ pH range of the studied wetlands. The PO assay is sensitive and activity could be detected with either substrate across a pH range of 4 to 7. However, with the standard enzyme tyrosinase, it was shown that a large change or threshold in oxidation rates occurred at pH 5. At pH < 5, L-DOPA oxidation rates were greatly diminished and ABTS oxidation was at a maximum. Above pH 5, ABTS oxidation occurred at much slower rates and L-DOPA oxidation was at a maximum. The pH response of PO activity in wetland soils corroborated observations made with tyrosinase. Thus, ABTS is recommended to be an effective substrate for the quantification of PO activity at an in situ pH of < 5, while L-DOPA is recommended at an in situ pH of > 5. In soils collected from a northern Minnesota peatland, assays conducted at an in situ pH of 4 showed one to two orders of magnitude higher rates of PO activity in solid phase peat in comparison to porewater, indicating that the majority of PO activity is associated with the peat. At three Minnesota peatland sites, PO activity was shown to attenuate with depth in agreement with the activities of other enzymes and with rates of peat decomposition.

Phenol oxidase

Wetland

Peatland

The influence of surface-active agents on the activity of tyrosinase and catalase ...

Tenenbaum, Leon Edward,

January 1940

Thesis (Ph. D.)--Columbia University, 1942. / Vita. Bibliography: p. 22.

Catalase. Phenol oxidase.

A study of the oxidation of catechol in the presence of tyrosinase

Wagreich, Harry,

January 1938

Thesis (Ph. D.)--Columbia University, 1938. / Vita.

Oxidation. Catechol. Phenol oxidase.

The tyrosine-tyrosinase reaction and its relation to plant respiration,

Robinson, Eugene Sant, Nelson, John Maurice,

January 1900

Thesis (Ph. D.)--Columbia University, 1945. / "Lithoprinted." Vita. Bibliography: p. 19.

Phenol oxidase. Plants

On the inactivation of the catecholase activity of tyrosinase during the enzymatic oxidation of certain substituted catechols

Roth, Lloyd J.

January 1944

Diss. - Columbia University.

Catechol. Phenol oxidase.

The kinetics of the reaction inactivation of tyrosinase during its catalysis of the aerobic oxidation of catechol

Asimov, Isaac,

January 1948

Thesis--Columbia University. / Vita. Bibliography: p. 65-66.

Phenol oxidase. Catechol.

On the mechanism of the reaction involved in the aerobic oxidation of catechol when catalyzed by the enzyme, tyrosinase ...

Soloway, Saul,

January 1941

Thesis (Ph. D.)--Columbia University, 1942. / Vita. Bibliography: p. 14.

Catechol. Oxidation. Phenol oxidase.

The oxidation of catechol-type substrates by tyrosinase

Cushing, Merchant Leroy,

January 1941

Thesis (Ph. D.)--Columbia University, 1941. / Vita. Bibliography: p. 20.

Catechol. Oxidation. Phenol oxidase.