Immobilization of snailase and β-glucosidase on L-aspartic acid-modified magnetic amorphous ZIF for efficiently and sustainably producing ginsenoside compound K.

Int J Biol Macromol

School of Environmental and Chemical Engineering, Xi'an Key Laboratory of Textile Chemical Engineering Auxiliaries, Engineering Research Center of Biological Resources Development and Pollution Control Universities of Shaanxi Province, Key Laboratory of Textile Dyeing Wastewater Treatment Universities of Shaanxi Province, Xi'an Polytechnic University, Xi'an 710048, PR China. Electronic address:

Published: December 2024

Improving the catalytic efficiency and recyclability of immobilized enzyme remained a serious challenge in industrial applications. Enzyme immobilization in the amorphous zeolite imidazolate framework (aZIF) preserved high enzyme activity, but still faced separation difficulties and a low catalytic efficiency in practice. In this study, a one-pot co-precipitation method was used to form the enzyme-aZIF/magnetic nanoparticle (MNP) biocomposite by rapidly precipitating snailase (Sna) and β-glucosidase (β-G) with metal/ligand on MNP and modifying with L-aspartic acid (Asp). Thanks to Asp modification protecting the natural conformation of internal protein molecules and MNP stabilizing the conformation of active enzymes after immobilizing, Sna&β-G in the carrier had more stable conformations and higher catalytic efficiency than those in conventional ZIF-8, increasing the catalytic efficiency for converting ginsenoside Rb1 to rare ginsenoside compound K (CK) to 79.16 %. Moreover, while improving the stability of Sna&β-G, owing to the magnetism imparted by MNP, the immobilized enzyme maintained high enzyme activity and recovery after 7 cycles by rapid magnetic separation. The results provided guidance for developing immobilized Sna&β-G biocomposites with ideal catalytic efficiency and easy recovery to catalyze ginsenoside Rb1 to rare ginsenoside CK.

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Source
http://dx.doi.org/10.1016/j.ijbiomac.2024.139230DOI Listing

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