A novel hybrid biocatalyst from immobilized Eversa® Transform 2.0 lipase and its application in biolubricant synthesis

被引:19
|
作者
de Sousa, Isamayra Germano [1 ]
Chaves, Anderson Valerio [2 ]
Barros de Oliveira, Andre Luiz [3 ]
Moreira, Katerine da Silva [3 ]
de Sousa Junior, Paulo Goncalves [4 ]
Neto, Francisco Simao [1 ]
Freitas de Carvalho, Simone Cristina [1 ]
Rodrigues Valerio, Roberta Bussons [2 ]
Lima, Gledson Vieira [4 ]
Sanders Lopes, Ada Amelia [1 ]
Martins de Souza, Maria Cristiane [1 ]
da Fonseca, Aluisio Marques [5 ]
Almeida Fechine, Pierre Basilio [2 ]
de Mattos, Marcos Carlos [4 ]
dos Santos, Jose C. S. [1 ]
机构
[1] Univ Integracao Int Lusofonia Afro Brasileira, Inst Engn & Desenvolvimento Sustentavel, Redencao, Brazil
[2] Univ Fed Ceara, Dept Quim Analit & Fis Quim, Fortaleza, Ceara, Brazil
[3] Univ Fed Ceara, Dept Engn Quim, Fortaleza, Ceara, Brazil
[4] Univ Fed Ceara, Dept Quim Organ & Inorgan, Fortaleza, Ceara, Brazil
[5] Univ Integracao Int Lusofonia Afro Brasileira, Sociobiodiversidades & Tecnol Sustentaveis MASTS, Inst Engn & Desenvolvimento Sustentavel, Acarape, CE, Brazil
关键词
Eversa (R) Transform 2.0; enzymatic immobilization; chitosan; agarose; biolubricants; docking studies; ENZYME IMMOBILIZATION; COVALENT IMMOBILIZATION; THERMOMYCES-LANUGINOSUS; INDUSTRIAL BIOCATALYSTS; CANDIDA-ANTARCTICA; KINETIC RESOLUTION; ACTIVATED AGAROSE; TAGUCHI DESIGN; GLUTARALDEHYDE; BIODIESEL;
D O I
10.1080/10242422.2022.2144263
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
In this study, a Taguchi experimental design was used for optimzing the immobilization of the lipase Eversa (R) Transform 2.0 (EVS) onto a hybrid support consisting of chitosan (CHI) and agarose (AGA), with glutaraldehyde (GLU) used as the support activator. The biocatalyst obtained was characterized by X-Ray Diffraction (XRD), Fourier Transform Infrared Spectroscopy (FTIR), Thermogravimetry (TGA), Energy Dispersive Spectroscopy (EDS), and Scanning Electron Microscopy (SEM). The optimized reaction conditions (60 min, 5 mM ionic strength, 1% GLU concentration, and 5 mg protein load per g of support) resulted in a highly active biocatalyst (74.39 +/- 0.48 U/g) and delivered an immobilization yield of 74.20 +/- 0.28%. The biocatalyst produced was observed to lose only 15.3% of its activity after 61 days of storage. The activity was also observed to increase by 96.70% +/- 0.76, 27.34% +/- 2.34, and 84.35% +/- 1.68 in the presence of the organic solvents hexane, cyclohexane, and methanol, respectively. Additionally, the byocatalist showed more pronounced activity at temperatures above 50 degrees C and was still able to retain approximately 30% of it at 70 degrees C. These values were found to be higher at alkaline pHs, as the activity of Eversa (R) 2.0 Transform saw an increase of up to 140% at pH 9. The desorption tests performed did not reveal any enzymatic detachment from the support. The novel biocatalyst also showed promising ester-lubricating properties. Furthermore, the in silico study revealed a binding affinity of -5.1 kcal/mol between oleic acid and the enzyme, suggesting that the combination of the substrate and the lipase was more stable and therefore, suitable for esterification. [GRAPHICS] .
引用
收藏
页码:151 / 172
页数:22
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