Exploring the Model of Cefazolin Released from Jellyfish Gelatin-Based Hydrogels as Affected by Glutaraldehyde

Author:

Charoenchokpanich Wiriya1ORCID,Muangrod Pratchaya1,Roytrakul Sittiruk2ORCID,Rungsardthong Vilai134,Wonganu Benjamaporn5,Charoenlappanit Sawanya2,Casanova Federico6ORCID,Thumthanaruk Benjawan134

Affiliation:

1. Department of Agro-Industrial, Food, and Environmental Technology, Faculty of Applied Science, King Mongkut’s University of Technology North Bangkok, Bangkok 10800, Thailand

2. Functional Proteomics Technology Laboratory, National Science and Technology Development Agency (NSTDA), Pathum Thani 12120, Thailand

3. Food and Agro-Industry Research Center, King Mongkut’s University of Technology North Bangkok, Bangkok 10800, Thailand

4. Center for Food Industry Innovation Technology, King Mongkut’s University of Technology North Bangkok, Bangkok 10800, Thailand

5. Department of Biotechnology, Faculty of Applied Science, King Mongkut’s University of Technology North Bangkok, Bangkok 10800, Thailand

6. Research Group for Food Production Engineering, National Food Institute, Technical University of Denmark, 28000 Kongens Lyngby, Denmark

Abstract

Due to its excellent biocompatibility and ease of biodegradation, jellyfish gelatin has gained attention as a hydrogel. However, hydrogel produced from jellyfish gelatin has not yet been sufficiently characterized. Therefore, this research aims to produce a jellyfish gelatin-based hydrogel. The gelatin produced from desalted jellyfish by-products varied with the part of the specimen and extraction time. Hydrogels with gelatin: glutaraldehyde ratios of 10:0.25, 10:0.50, and 10:1.00 (v/v) were characterized, and their cefazolin release ability was determined. The optimal conditions for gelatin extraction and chosen for the development of jellyfish hydrogels (JGel) included the use of the umbrella part of desalted jellyfish by-products extracted for 24 h (WU24), which yielded the highest gel strength (460.02 g), viscosity (24.45 cP), gelling temperature (12.70 °C), and melting temperature (22.48 °C). The quantities of collagen alpha−1(XXVIII) chain A, collagen alpha−1(XXI) chain, and collagen alpha−2(IX) chain in WU24 may influence its gel properties. Increasing the glutaraldehyde content in JGel increased the gel fraction by decreasing the space between the protein chains and gel swelling, as glutaraldehyde binds with lateral amino acid residues and produces a stronger network. At 8 h, more than 80% of the cefazolin in JGel (10:0.25) was released, which was higher than that released from bovine hydrogel (52.81%) and fish hydrogel (54.04%). This research is the first report focused on the production of JGel using glutaraldehyde as a cross-linking agent.

Funder

King Mongkut’s University of Technology North Bangkok and National Science and Technology Development Agency

National Research Council of Thailand through the NRCT Senior Research Scholar Program

Publisher

MDPI AG

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