Abstract
Summary
Biomass of the fungus Fusarium proliferatiim was produced and used to obtain a crude extract (FI) of lipoxygenase. The enzyme was further purified by ammonium sulfate precipitation at 40% of saturation (FII). The enzymatic extract (FII) showed its optimum activity at pH 6.0. The apparent K m and V max values for the lipoxygenase (FII) were calculated to be 5.15 × 10−5 M and 1.61 μmol hydroperoxide/mg protein/min, respectively. Enzyme activity remained relatively stable at potassium cyanide concentrations as high as 60 mM. The presence of 5 mM ethylenediaminetetraacetate activated the enzyme by 50%, whereas the use of 1.2 mM hydroquinone resulted in a 2‐fold increase in lipoxygenase activity. The partially purified enzyme (FII) showed a three‐fold enhancement of activity towards linoleic acid compared to linolenic acid as well as mono‐, di‐ and trilinolein.