Purification of Glucose Oxidase and Catalase Produced by the Apple Blue Mold, Penicillium expansum O-385-10, and Their Characteristics Including the Browning of Apple Fruit

Hyun-Woong KIM; Soichiro KIMURA; Nobuko OHNO; Miho OKADOME; Haruo TAKAHASHI; Seigo AMACHI; Hirofumi SHINOYAMA; Takaaki FUJII

doi:10.5803/jsfm.22.10

Purification of Glucose Oxidase and Catalase Produced by the Apple Blue Mold, Penicillium expansum O-385-10, and Their Characteristics Including the Browning of Apple Fruit

Hyun-Woong KIM, Soichiro KIMURA, Nobuko OHNO, Miho OKADOME, Haruo TAKAHASHI, Seigo AMACHI, Hirofumi SHINOYAMA, Takaaki FUJII

Author information

Hyun-Woong KIM
Department of Life and Bioresources Science, Graduate School of Science and Technology, Chiba University
Soichiro KIMURA
Department of Life and Bioresources Science, Graduate School of Science and Technology, Chiba University
Nobuko OHNO
Department of Health and Nutrition, School of Home Economics, Wayo Women's University
Miho OKADOME
Department of Health and Nutrition, School of Home Economics, Wayo Women's University
Haruo TAKAHASHI
Public Health Laboratory of Chiba Prefecture
Seigo AMACHI
Department of Life and Bioresources Science, Graduate School of Science and Technology, Chiba University
Hirofumi SHINOYAMA
Department of Life and Bioresources Science, Graduate School of Science and Technology, Chiba University
Takaaki FUJII
Department of Life and Bioresources Science, Graduate School of Science and Technology, Chiba University

Keywords: Glucose oxidase, Catalase, Penicillium expansum, Apple fruit

JOURNAL FREE ACCESS

2005 Volume 22 Issue 1 Pages 10-16

DOI https://doi.org/10.5803/jsfm.22.10

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Abstract

Penicillium expansumO-385-10 produces glucose oxidase and catalase but showed poorgrowth in medium containing glucose as a sole carbon source. In this culture, gluconate wasaccumulated, the pH of the culture medium decreased during incubation, and growth wasremarkably inhibited. Glucose oxidase and catalase were purified as electrophoreticallyhomogeneous proteins from the culture in which the pH was adjusted using calcium carbonate.The molecular weights of glucose oxidase and catalase were estimated at about 130 kDa (homodimer) and 300 kDa (homotetramer). Glucose oxidase and catalase showed about 80%and 50% activity at pH 3, respectively. The catalase was remarkably activated by 1mM Ca²⁺and 1mM Ba²⁺. When glucose oxidase and catalase were simultaneously incubated withsmall pieces of apple, the fruit tissue browned remarkably. No browning reaction occurredwhen each enzyme was incubated independently.

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