Purification, characterization, gene cloning and sequencing of a new β-glucosidase from Aspergillus niger BE-2
- Authors: Ali N.1,2, Xue Y.3, Gan L.3, Liu J.3, Long M.3
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Affiliations:
- School of Life Science
- Department of Biochemistry
- College of Energy
- Issue: Vol 52, No 5 (2016)
- Pages: 564-571
- Section: Article
- URL: https://journal-vniispk.ru/0003-6838/article/view/152049
- DOI: https://doi.org/10.1134/S0003683816050045
- ID: 152049
Cite item
Abstract
The cDNA gene (BgL1), encoding GH3 family β-glucosidase (EC 3.2.1.21) from Aspergillus niger BE-2 (abbreviated to BgL1), was amplified and inserted into the yeast expression pPIC9K vector at the site of Bln I (Avr II) and NotI. The recombinant expression vector, designated as pPIC9K-BgL1, was transformed into Pichia pastoris GS115. The transformants were screened on minimal dextrose plates, which inoculated on geneticin G418-containing yeast extract-peptone-dextrose plates. The transformants expressed the high β-glucosidase activity of 22.6 U/mL. SDS-PAGE demonstrated that the BgL1 was extracellularly expressed with an apparent molecular weight of 90.0 kDa. The purified BgL1 displayed the maximum activity at pH 6.0 and 60°C. It was highly stable at a broad pH range of 4.0–7.5 and temperature of 60°C. The BgL1 displayed high similarity to the β-glucosidases of A. niger FN430671 and A. niger DQ655704, the members of the GH3 family. Its three-dimensional structure was predicted using http://swiss-model.expasy.org/ on-line programs based on the crystal structure of Aspergillus aculeatus β-glucosidase.
About the authors
N. Ali
School of Life Science; Department of Biochemistry
Email: jianliu@xmu.edu.cn
China, Xiamen, 361005; Mardan, 23200
Y. Xue
College of Energy
Email: jianliu@xmu.edu.cn
China, Xiamen, 361005
L. Gan
College of Energy
Email: jianliu@xmu.edu.cn
China, Xiamen, 361005
J. Liu
College of Energy
Author for correspondence.
Email: jianliu@xmu.edu.cn
China, Xiamen, 361005
M. Long
College of Energy
Email: jianliu@xmu.edu.cn
China, Xiamen, 361005
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