Optimization of protease production process using bran waste using Bacillus licheniformis

Protease enzyme production by Bacillus licheniformis bacteria was investigated. Various agricultural wastes as substrate such as wheat bran, rice bran, and sugarcane bagasse were considered. The most important effective parameters on enzyme production, like incubation time, various substrates and so...

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Bibliographic Details
Published in:The Korean journal of chemical engineering 2022, 39(3), 264, pp.674-683
Main Authors: Espoui, Amin Heydari, Larimi, Saeedeh Gilani, Darzi, Ghasem Najafpour
Format: Article
Language:English
Subjects:
Agricultural wastes
Bagasse
Bioreactors
Biotechnology
Catalysis
Chemistry
Chemistry and Materials Science
Cotton
Enzymes
Industrial Chemistry/Chemical Engineering
Materials Science
Optimization
Particle size
Peptones
Protease
Shelf life
Substrates
Sugarcane
Thermal stability
Wheat
화학공학
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Summary:Protease enzyme production by Bacillus licheniformis bacteria was investigated. Various agricultural wastes as substrate such as wheat bran, rice bran, and sugarcane bagasse were considered. The most important effective parameters on enzyme production, like incubation time, various substrates and solid substrate particle size, media pH, different nitrogen sources in a bench-scale designed bioreactor, were optimized. The optimum protease production conditions, for both Erlenmeyer flask and batch bioreactor, at 37 °C, pH of 8, incubation time of 48h, wheat bran (5 wt%) with the particle size of 1 mm, an equal amount of peptone and yeast extract (1% w/w) and agitation rate of 180 rpm were defined. In addition, maximum protease activity in the Erlenmeyer flask and batch bioreactor was 596 and 683.93 U/mL, respectively. The pH and thermal stability of produced protease were studied; the highest amount of remaining activities at pH 8 and 60 °C were 97 and 63% of initial activities, respectively. Also, shelf-life of the produced protease enzyme retained up to 88% of its initial activity after 30 days of storage at 4 °C. However, the produced enzyme was exposed remarkably compatible with the commercial detergent; the enzyme perfectly washed and removed the stains from the sample cotton textile.
ISSN:0256-1115
1975-7220
DOI:10.1007/s11814-021-0965-3