Method for the measurement of lipase activity in milk

GERARD HUMBERT; MARIE-FRANCE GUINGAMP; GUY LINDEN

doi:10.1017/S0022029997002288

Abstract

Lipolysis has many effects in dairy technology. Undesirable consequences include deleterious effects on the organoleptic properties of milk and some cheeses; however, it is desirable in some other cheeses.

The usual methods for detecting lipolysis in milk measure the amounts of free fatty acids liberated from triacylglycerols (International Dairy Federation, 1991). Lipase activity is detected by incubation of samples with substrates such as tributyrin (Castberg et al. 1975) or triolein (Nilsson-Ehle & Schotz, 1976; Shirai et al. 1982). A few reports describe methods using synthetic chromogenic substrates, e.g. p-nitrophenyl butyrate (Shirai & Jackson, 1982), β-naphthyl caprylate (McKellar, 1986; McKellar & Cholette, 1986) or 4-methylumbelliferyl oleate (Stead, 1983). Tsakalidou et al. (1992) have developed the detection of esterase activities on electrophoresis gels.

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Method for the measurement of lipase activity in milk

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