Study on the “Glutamic Acid-Enzymolysis” Process for Extracting Chitin from Crab Shell Waste and its By-Product Recovery

Chitin is the second-most abundant bioresource and widely used in the food, agricultural, biomedicine, and other industries. However, under the mutual restriction of extraction cost and environmental protection, it is relatively difficult to prepare chitin from natural sources by pure separation. Th...

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Bibliographic Details
Published in:Applied biochemistry and biotechnology 2020-03, Vol.190 (3), p.1074-1091
Main Authors: Ding, Huipu, Lv, Le, Wang, Zhijiang, Liu, Liping
Format: Article
Language:English
Subjects:
Alkaline protease
Amino acids
Animals
Bacteria
Bacterial Proteins - metabolism
Biochemistry
Biotechnology
Brachyura - chemistry
By products
Calcium - metabolism
Calcium carbonate
Calcium phosphates
Caustic soda
Chemistry
Chemistry and Materials Science
Chitin
Chitin - isolation & purification
Chitin - metabolism
Crustaceans
Decalcification
Deproteinization
Endopeptidases - metabolism
Environmental protection
Enzymes
Enzymolysis
Feed additives
Fermentation
Food additives
Glutamic acid
Glutamic Acid - metabolism
Hydrogen
Hydrogen-Ion Concentration
Polypeptides
Protease
Proteins
Proteolysis
Raw materials
Recovering
Temperature
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Summary:Chitin is the second-most abundant bioresource and widely used in the food, agricultural, biomedicine, and other industries. However, under the mutual restriction of extraction cost and environmental protection, it is relatively difficult to prepare chitin from natural sources by pure separation. The aim of this study is to extract chitin from fresh crab shell waste by decalcification (DC) and deproteinization (DP) using glutamic acid and alkaline protease. The optimum technological conditions for DC and DP were as follows: (1) 5% (w/v) glutamic acid solution was used as decalcifying agent, the ratio of material to liquid was 1:10 (m/v), and the ash content in chitin was 0.83 ± 0.027% after decalcification at 75° C for 12 h. (2) Using alkaline protease as enzymatic hydrolyzer, 1500 U of alkaline protease was added per gram of crab shell. Under the conditions of material-liquid ratio of 1:10 (m/v) and pH value of hydrolysate of 9.0, N content in chitin was 6.63 ± 0.10% after 6 h of enzymatic hydrolysis at 55° C. And the extraction rate of chitin was 92.25 ± 0.51%. As a decalcifying agent, glutamic acid could be recycled with a recovery rate of 77.42 ± 2.16%. Calcium carbonate in crab shell was converted into calcium hydrogen phosphate by calcium glutamate, and protein into amino acids and polypeptides, which could be used as feed additives. The “glutamic acid-enzymolysis” for extracting chitin from crab shell is a relatively closed process, which has the advantages of mild reaction, greatly reducing the discharge of three wastes and high comprehensive utilization rate of raw materials.
ISSN:0273-2289
1559-0291
DOI:10.1007/s12010-019-03139-2