Affiliation:
1. Institute of Biochemistry Department of Biotechnology and Enzyme Catalysis University of Greifswald Felix-Hausdorff-Straße 4 17487 Greifswald Germany
2. Institute of Molecular Biotechnology Graz University of Technology Petersgasse 14 8010 Graz Austria
3. Henkel AG & Co. KGaA Adhesive Research Henkelstraße 67 40191 Düsseldorf Germany
4. acib – Austrian Centre of Industrial Biotechnology Petersgasse 14 8010 Graz Austria
5. BioTechMed-Graz Mozartgasse 12/II 8010 Graz Austria
Abstract
AbstractBiocatalytic decarboxylation of hydroxycinnamic acids yields phenolic styrenes, which are important precursors for antioxidants, epoxy coatings, adhesives and other polymeric materials. Bacillus subtilis decarboxylase (BsPAD) is a cofactor‐independent enzyme that catalyzes the cleavage of carbon dioxide from p‐coumaric‐, caffeic‐, and ferulic acid with high catalytic efficiency. Real‐time spectroscopic assays for decarboxylase reactions remove the necessity of extensive sample workup, which is required for HPLC, mass spectrometry, gas chromatography, or NMR methods. This work presents two robust and sensitive assays based on photometry and fluorimetry that allow decarboxylation reactions to be followed with high sensitivity while avoiding product extraction and long analysis times. Optimized assay procedures were used to measure BsPAD activity in cell lysates and to determine the kinetic constants (KM and Vmax) of the purified enzyme for p‐coumaric‐, caffeic‐ and ferulic acid. Substrate inhibition was shown for caffeic acid.
Funder
Bundesministerium für Klimaschutz, Umwelt, Energie, Mobilität, Innovation und Technologie
Bundesministerium für Digitalisierung und Wirtschaftsstandort
Steirische Wirtschaftsförderungsgesellschaft
Standortagentur Tirol
Amt der NÖ Landesregierung
Subject
Organic Chemistry,Molecular Biology,Molecular Medicine,Biochemistry
Cited by
1 articles.
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