Winged bean lipoxygenase-Part 2: Physicochemical properties

Abstract

Winged bean lipoxygenase (linoleate: oxygen oxidoreductase EC 1.13.11.12) isoenzymes FI and FII were isolated and purified according to the method of Truong et al. (1980). FI and FII were both highly specific for linoleic acid. They exhibited optimal activity at pH 6·0 and 5·8, respectively at 30°C. An activation energy of 4·5 kcal mol-1 was calculated for this lipoxygenase within the temperature range of 30-50°C. At 0·075% Tween 20, FI and FII had Km values for linoleic acid of 0·44 and 0·37 × 10-3M, respectively, compared to 0·4 × 10-3M for the crude enzyme. Maximal activity was obtained at 1·6 × 10-3M. Higher levels of Tween 20 inhibited the lipoxygenase activity. Both isoenzymes had identical average molecular weight of 80 000 daltons by gel filtration and SDS gel electrophoresis. FI and FII isoenzymes were strongly inhibited by Hg++, Mn++, Mg++ and Fe+++ and activated by Zn++, Co++ and Fe++. A difference in the degree of inhibition or activation was observed between FI and FII response. Ca++ inhibited both FI and FII but the former was more sensitive to Ca++. KCN also inhibited the two isoenzymes. Among the antioxidants tested, butylated hydroxytoluene and butylated hydroxyanisole most effectively inhibited both FI and FII at only 10-6M. Sulphydryl reagents such as iodoacetamide and dithiothreitol have little effect on the lipoxygenase isoenzyme activity. The lipoxygenase isoenzymes were more stable at neutral pH. The enzyme in the crude extract and especially in situ was more stable to heat treatment. © 1982.

Source or Periodical Title

Food Chemistry

ISSN

3088146

Page

277-289

Document Type

Article

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