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Preparation and characteristics of squid pen β‐chitin prepared under optimal deproteinisation and demineralisation condition
Authors:Dal Kyoung Youn  Hong Kyoon No  Witoon Prinyawiwatkul
Affiliation:1. Department of Food Science and Technology, Catholic University of Daegu, , Hayang, 712‐702 South Korea;2. Department of Food Science, Louisiana State University Agricultural Center, , Baton Rouge, LA, 70803‐4200 USA
Abstract:Squid (Todarodes pacifica) pen was an excellent source of β‐chitin with 25.5% yield. The optimal condition to prepare squid pen β‐chitin was established: deproteinisation with 3% NaOH for 30 min at 15 psi/121 °C and a solid/solvent ratio of 1:10 (w/v) and a subsequent demineralisation with 1 N HCl for 30 min at room temperature and a solid/solvent ratio of 1:10 (w/v). Squid pen β‐chitin contained 6.29% nitrogen, 0.25% ash, and negligible fat with degree of acetylation of 94.02%, residual amino acid of 0.499 g/100 g and bulk density of 0.28 g mL?1. Depending on its particle size, squid pen β‐chitin visually looked white (L* = 82.82, a* = ?0.67, b* = 6.31; particle size of 0.15–0.18 mm) or light grey (L* = 62.88, a* = 0.33, b* = 10.66; particle size of 0.425–0.841 mm). Water, fat and dye‐binding capacity of squid pen β‐chitin was 694.67%, 194.03% and 79.81%, respectively.
Keywords:Binding capacity  chitin  demineralisation  deproteinisation  squid pen
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