Optimization of Aspergillus niger NRC1ami Pectinase Using Citrus Peel Pectin, Purification, and Thermodynamic Characterization of the Free and Modified Enzyme

被引:11
|
作者
Esawy, Mona A. [1 ]
Gamal, Amira A. [1 ]
Kamel, Zeinat [1 ]
机构
[1] Natl Res Ctr, Pharmaceut Ind Res Inst, Chem Nat & Microbial Prod Dept, Cairo, Egypt
关键词
Fungi; Pectinase; Citrus peel; Purification; Modification; Thermodynamic; SOLID-STATE FERMENTATION; COMPLEX; YEAST;
D O I
10.1007/s12649-022-01838-2
中图分类号
X [环境科学、安全科学];
学科分类号
08 ; 0830 ;
摘要
Enzyme cost and stability are the main problems facing industrial applications. Consequently, Aspergillus nigerNRC1ami was isolated from rotten orange and recorded a promising pectinase activity (13.8 U/ml). The enzyme was optimized using citrus peel pectin as the sole carbon source and recorded (40 U/ml). It was purified by two steps purifications and recorded 632 purification folds. The pure enzyme showed 14.7% carbohydrate content and consists of 15 amino acids. Glutamic acid was the major (22%) followed by leucine (10.67%) and threonine was the minor (2.70%). A. niger NRC1ami pectinase was conjugated by covalent coupling to sodium periodate (NaIO4) activated polysaccharides. Galactomannan showed the highest recovered activity (85%) and 94.34% reduction in viscosity. The optimum temperature for the pure enzyme shifted from 40 to 45 degrees C after the conjugation process. Also, the free enzyme showed its optimum activity at pH 5 compared to pH 4, 5 in the conjugated form case. The thermal stability of the free enzyme greatly improved after the modification process. The conjugated process reduced the activation energy to 36%, prolonged the enzyme half-life 5.6-fold at 60 degrees C, and increase the deactivation energy (Ed) by about 19% in comparison to the free form. The D value of the conjugated enzyme increased to 13.2-fold at 50 degrees C compared to the free form. Gibbs's free energy (Delta G) of the enzyme increased after the modification process, while the enthalpy (Delta H) and entropy (Delta S) decreased. Na+ and Zn2+ had a stimulating effect on both enzyme forms. [GRAPHICS] .
引用
收藏
页码:4823 / 4837
页数:15
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