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Merck
  • Fluorescent inhibitors for the qualitative and quantitative analysis of lipolytic enzymes.

Fluorescent inhibitors for the qualitative and quantitative analysis of lipolytic enzymes.

Analytical biochemistry (1999-12-10)
H Scholze, H Stütz, F Paltauf, A Hermetter
摘要

We report on the determination of active enzyme components in pure and crude lipases, using fluorescent inhibitors for covalent modification and visualization of the enzymatically active proteins. Lipase-specific compounds are triacylglycerol analogs, namely 1,2(2, 3)-di-O-alkylglyceroalkylphosphonic acid-p-nitrophenyl esters, containing a fluorescent substituent bound to the omega-end of an alkyl chain. Inhibitors derived from single-chain alcohols, such as p-nitrophenyl esters of fluorescent alkyl phosphonates, react with lipases and esterases. The p-nitrophenyl ester bond is susceptible toward nucleophilic attack by the active serine of the lipolytic enzyme. This reaction is stoichiometric, specific, and irreversible. Stable lipid-protein complexes are formed which can be analyzed on the basis of their fluorescent signal. From fluorescence intensity the moles of active serine (enzyme) were accurately determined. A lipase-specific inhibitor was used for the analysis of a commercial lipase preparation from Rhizomucor miehei. After incubation of the enzyme with the fluorescent lipid, a single fluorescence band was observed after SDS-gel electrophoresis, indicating the presence of a single lipase in the crude enzyme material. A linear correlation was obtained between fluorescence intensity and the amount of enzyme. Using a combination of different inhibitors, we were able to discriminate between lipases and esterases.

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脂肪酶 来源于黑曲霉, powder (fine), ~200 U/g
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脂肪酶 来源于小麦胚芽, Type I, lyophilized powder, 5-15 units/mg solid
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脂肪酶底物, ≥95% (HPLC)
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脂肪酶 来源于米根霉, powder (fine), ~10 U/mg
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Lipase Substrate, for the titrimetric determination of enzyme activity