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Immobilized lipoxygenase in continuous production of fatty acid hydroperoxides
Author(s) -
Laakso Simo
Publication year - 1982
Publication title -
lipids
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.601
H-Index - 120
eISSN - 1558-9307
pISSN - 0024-4201
DOI - 10.1007/bf02534648
Subject(s) - chemistry , lipoxygenase , chromatography , substrate (aquarium) , agarose , immobilized enzyme , linoleic acid , fatty acid , covalent bond , catalysis , enzyme , biochemistry , organic chemistry , geology , oceanography
Abstract Soybean lipoxygenase‐1 was covalently coupled to agarose with 75% recovery of catalytic activity. Because evidence was obtained that the immobilization resulted in improved operational stability of the enzyme, a lipoxygenase‐reactor and a continuous process for the synthesis of 13‐hydroperoxy‐linoleic acid and 15‐hydroperoxyarachidonic acid were developed. A procedure based on spectrophotometric hydroperoxide assay and constant oxygraphic monitoring of the effluent is presented for the calibration of the reactor to operate at the highest conversion efficiency when oxygenating quantitatively the substrate. Under these conditions, the reactor was capable of producing about 0.6 mg of hydroperoxy fatty acid/1.0 ml of wet gel/hr. The covalently coupled enzyme has been stable during six months of storage at 3 C in 0.2 M Na‐borate buffer, pH 9.0, and during the same period, its operational stability in the column has been unaltered under the conditions used.