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Glucuronoyl Esterase Screening and Characterization Assays Utilizing Commercially Available Benzyl Glucuronic Acid Ester.

Molecules (Basel, Switzerland) (2015-09-26)
Hampus Sunner, Maria-Despoina Charavgi, Lisbeth Olsson, Evangelos Topakas, Paul Christakopoulos
RÉSUMÉ

Research on glucuronoyl esterases (GEs) has been hampered by the lack of enzyme assays based on easily obtainable substrates. While benzyl d-glucuronic acid ester (BnGlcA) is a commercially available substrate that can be used for GE assays, several considerations regarding substrate instability, limited solubility and low apparent affinities should be made. In this work we discuss the factors that are important when using BnGlcA for assaying GE activity and show how these can be applied when designing BnGlcA-based GE assays for different applications: a thin-layer chromatography assay for qualitative activity detection, a coupled-enzyme spectrophotometric assay that can be used for high-throughput screening or general activity determinations and a HPLC-based detection method allowing kinetic determinations. The three-level experimental procedure not merely facilitates routine, fast and simple biochemical characterizations but it can also give rise to the discovery of different GEs through an extensive screening of heterologous Genomic and Metagenomic expression libraries.

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Alcool benzylique, ReagentPlus®, ≥99%
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Alcool benzylique, ACS reagent, ≥99.0%
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Alcool benzylique, puriss., meets analytical specification of Ph. Eur., BP, NF, 99-100.5% (GC)
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Alcool benzylique, puriss. p.a., ACS reagent, ≥99.0% (GC)
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Alcool benzylique, ≥99%, FCC, FG
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Alcool benzylique, anhydrous, 99.8%
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Alcool benzylique, natural, ≥98%, FG