Comparison of Free and Immobilized L-asparaginase Synthesized by Gamma-Irradiated Penicillium cyclopium

Gamma irradiation is used on Penicillium cyclopium in order to obtain mutant cells of high L-asparaginase productivity. Using gamma irradiation dose of 4 KGy, P. cyclopium cells yielded L-asparaginase with extracellular enzyme activity of 210.8 ± 3 U/ml, and specific activity of 752.5 ± 1.5 U/mg pro...

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Bibliographic Details
Published in:Polish journal of microbiology 2016-01, Vol.65 (1), p.43-50
Main Authors: El-Refai, Heba A, Shafei, Mona S, Mostafa, Hanan, El-Refai, Abdel-Monem H, Araby, Eman M, El-Beih, Fawkia M, Easa, Saadia M, Gomaa, Sanaa K
Format: Article
Language:English
Subjects:
Acetone
Amberlite (trademark)
Ammonia
Asparaginase
Asparaginase - genetics
Asparaginase - metabolism
Cancer therapies
Cellulose
Enzymatic activity
Enzyme activity
Enzymes
Enzymes, Immobilized - metabolism
Free form
Fungi
Gamma irradiation
Gene Expression Regulation, Enzymologic - radiation effects
Gene Expression Regulation, Fungal - radiation effects
High temperature
Hydrogen-Ion Concentration
Immobilization
Immobilized enzymes
Irradiation
Kinetics
L-asparaginase
Leukemia
Metals
Mutation
Penicillium
Penicillium - enzymology
Penicillium - radiation effects
pH effects
Polyvinyl alcohol
Precipitation (Meteorology)
Proteins
Radiation dosage
Thermal stability
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Summary:Gamma irradiation is used on Penicillium cyclopium in order to obtain mutant cells of high L-asparaginase productivity. Using gamma irradiation dose of 4 KGy, P. cyclopium cells yielded L-asparaginase with extracellular enzyme activity of 210.8 ± 3 U/ml, and specific activity of 752.5 ± 1.5 U/mg protein, which are 1.75 and 1.53 times, respectively, the activity of the wild strain. The enzyme was partially purified by 40-60% acetone precipitation. L-asparaginase was immobilized onto Amberlite IR-120 by ionic binding. Both free and immobilized enzymes exhibited maximum activity at pH 8 and 40 degrees C. The immobilization process improved the enzyme thermal stability significantly. The immobilized enzyme remained 100% active at temperatures up to 60 degrees C, while the free asparaginase was less tolerant to high temperatures. The immobilized enzyme was more stable at pH 9.0 for 50 min, retaining 70% of its relative activity. The maximum reaction rate (V(max)) and Michaelis-Menten constant (K(m)) of the free form were significantly changed after immobilization. The K(m) value for immobilized L-asparaginase was about 1.3 times higher than that of free enzyme. The ions K+, Ba2+ and Na+ showed stimulatory effect on enzyme activity with percentages of 110%, 109% and 106% respectively.
ISSN:1733-1331
2544-4646
DOI:10.5604/17331331.1197274