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Title: | Purification and physicochemical characterisation of Aspergillus niger USM F4 β-mannanase | Authors: | Syarifah, A.R. Darah, I. Ibrahim, C.O. Ramli, H. Tong, W.Y. |
Keywords: | Mannanase;palm kernel cake;physicochemical characterisation;protein purification | Issue Date: | 2020 | Publisher: | Universiti Sains Malaysia | Journal: | Malaysian Journal of Microbiology | Abstract: | This present study focused on purification of fungal β-mannanase produced by Aspergillus niger USM F4 and also physicochemical characterisation of the purified enzyme. Methodology and results: The purified β-mannanase with a molecular mass of ~47.4 kDa was demonstrated on SDS-PAGE gel. The enzyme signified a purification degree of 4-fold, with final specific activity of 196.42 U/mg. It reached an optimum catalytic activity at pH 4.0 and 60 °C. The thermal stability of the enzyme was up to 70 °C and maintained the 50% activity after 30 min at 80 °C. Meanwhile, the pH stability was in the range of pH 3.0-9.0 and a 30 min half-life at pH 10.0. All chemical substances manifested an inhibitory effect on purified β-mannanase, with SDS (28.16 ± 0.05% residual activity) as the strongest inhibitor, followed by cupric ion (Cu2+) (49.51 ± 0.09% residual activity). As a whole, the enzyme displayed a substrate specificity in the order of locust bean gum (LBG) > carboxymethylcellulose > soluble starch > xylan from oat spelt > α-cellulose. Its preference for LBG has generated the Km and Vmax values of 0.20 mg/mL and 9.82 U/mL, respectively. Conclusion, significance and impact of study: The outcomes of our study offer potential for use at industrial scales, particularly in the oligosaccharides production that involve acid-related activity, wide-ranging temperature and pH stability. |
Description: | Scopus |
URI: | http://hdl.handle.net/123456789/548 | ISSN: | 22317538 | DOI: | 10.21161/mjm.200719 |
Appears in Collections: | Faculty of Bioengineering and Technology - Journal (Scopus/WOS) |
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