Production of a Fungal Punicalagin-Degrading Enzyme by Solid-State Fermentation: Studies of Purification and Characterization

Pedro Aguilar-Zárate; Gerardo Gutiérrez-Sánchez; Mariela R. Michel; Carl W. Bergmann; José J. Buenrostro-Figueroa; Juan A. Ascacio-Valdés; Juan C. Contreras-Esquivel; Cristóbal N. Aguilar

doi:10.3390/foods12040903

Foods (Feb 2023)

Production of a Fungal Punicalagin-Degrading Enzyme by Solid-State Fermentation: Studies of Purification and Characterization

Pedro Aguilar-Zárate,
Gerardo Gutiérrez-Sánchez,
Mariela R. Michel,
Carl W. Bergmann,
José J. Buenrostro-Figueroa,
Juan A. Ascacio-Valdés,
Juan C. Contreras-Esquivel,
Cristóbal N. Aguilar

Affiliations

Pedro Aguilar-Zárate: Engineering Department, Instituto Tecnológico de Ciudad Valles, Tecnológico Nacional de México, Ciudad Valles, San Luis Potosí C.P. 79010, Mexico
Gerardo Gutiérrez-Sánchez: Complex Carbohydrate Research Center, The University of Georgia, Athens, GA 30602, USA
Mariela R. Michel: Engineering Department, Instituto Tecnológico de Ciudad Valles, Tecnológico Nacional de México, Ciudad Valles, San Luis Potosí C.P. 79010, Mexico
Carl W. Bergmann: Complex Carbohydrate Research Center, The University of Georgia, Athens, GA 30602, USA
José J. Buenrostro-Figueroa: Research Center in Food and Development A. C. Cd., Delicias, Chihuahua C.P. 33089, Mexico
Juan A. Ascacio-Valdés: Bioprocesses Research Group, Food Research Department, School of Chemistry, Universidad Autónoma de Coahuila, Saltillo, Coahuila C.P. 25280, Mexico
Juan C. Contreras-Esquivel: Bioprocesses Research Group, Food Research Department, School of Chemistry, Universidad Autónoma de Coahuila, Saltillo, Coahuila C.P. 25280, Mexico
Cristóbal N. Aguilar: Bioprocesses Research Group, Food Research Department, School of Chemistry, Universidad Autónoma de Coahuila, Saltillo, Coahuila C.P. 25280, Mexico

DOI: https://doi.org/10.3390/foods12040903
Journal volume & issue: Vol. 12, no. 4
p. 903

Abstract

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The present work describes the purification of an enzyme capable of degrading punicalagin. The enzyme was produced by Aspergillus niger GH1 by solid-state fermentation, and the enzyme production was induced by using ellagitannins as the sole carbon source. The purification steps included the concentration by lyophilization, desalting, anionic exchange, and gel filtration chromatography. The enzyme kinetic constants were calculated by using punicalagin, methyl gallate, and sugar beet arabinans. The molecular mass of the protein was estimated by SDS-PAGE. The identified bands were excised and digested using trypsin, and the peptides were submitted to HPLC-MS/MS analysis. The docking analysis was conducted, and a 3D model was created. The purification fold increases 75 times compared with the cell-free extract. The obtained Km values were 0.053 mM, 0.53% and 6.66 mM for punicalagin, sugar beet arabinans and methyl gallate, respectively. The optimal pH and temperature for the reaction were 5 and 40 °C, respectively. The SDS-PAGE and native PAGE analysis revealed the presence of two bands identified as α-l-arabinofuranosidase. Both enzymes were capable of degrading punicalagin and releasing ellagic acid.

Published in Foods

ISSN: 2304-8158 (Online)
Publisher: MDPI AG
Country of publisher: Switzerland
LCC subjects: Technology: Chemical technology
Website: http://www.mdpi.com/journal/foods

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