Home / Biochemistry / PRODUCTION OF PROTEASE BY ASPERGILLUS FLAVUS IN SOLID STATE FERMENTATION

PRODUCTION OF PROTEASE BY ASPERGILLUS FLAVUS IN SOLID STATE FERMENTATION

 

Table Of Contents


Chapter ONE

1.1 Introduction
1.2 Background of Study
1.3 Problem Statement
1.4 Objective of Study
1.5 Limitation of Study
1.6 Scope of Study
1.7 Significance of Study
1.8 Structure of the Research
1.9 Definition of Terms

Chapter TWO

2.1 Overview of Enzymes
2.2 Protease Enzyme: Types and Functions
2.3 Production of Protease Enzyme
2.4 Aspergillus Flavus: Characteristics and Applications
2.5 Solid State Fermentation: Process and Advantages
2.6 Factors Affecting Enzyme Production in Solid State Fermentation
2.7 Previous Studies on Protease Production by Aspergillus Flavus
2.8 Enzyme Purification Techniques
2.9 Enzyme Immobilization Methods
2.10 Industrial Applications of Protease Enzyme

Chapter THREE

3.1 Research Methodology Overview
3.2 Selection of Aspergillus Flavus Strain
3.3 Substrate Selection for Solid State Fermentation
3.4 Inoculum Preparation and Inoculation
3.5 Optimization of Solid State Fermentation Conditions
3.6 Enzyme Extraction and Purification Process
3.7 Enzyme Assay Methods
3.8 Data Analysis Techniques

Chapter FOUR

4.1 Analysis of Enzyme Production Results
4.2 Effect of Parameters on Protease Production
4.3 Comparison with Previous Studies
4.4 Enzyme Purification Results
4.5 Enzyme Characterization Data
4.6 Immobilization Efficiency and Stability
4.7 Industrial Scale-up Considerations
4.8 Discussion on Future Research Directions

Chapter FIVE

5.1 Summary of Findings
5.2 Discussion of Results
5.3 Conclusion and Implications
5.4 Recommendations for Further Research
5.5 Contribution to the Field

Project Abstract

The study for the production of protease from Aspergillus flavus using wheat bran as substrate under Solid State Fermentation was conducted in University of Abuja, Department of Microbiology. Aspergillus flavus was isolated from spoilt bread and was identified on the basis of the morphological assessment such as macroscopic and microscopy. Among the characteristics used includes colonial characteristics such surface appearance, texture and colour of the colonies. The protease activity increased with increase in the fermentation periods. The quantities of the protease enzyme produced by the Aspergillus flavus in the basal medium were measured using UV-Spectrophotometer and the result is shown in Table 5. The protease activity was found to be higher at day 7 than day 5 and 3 with 4.51±10.06 proteaase Unit/mL, 8.63±0.12 U/mL and 18.93±1.20 AU/mL respectively. the extracellular protease produced by Aspergillus flavus isolated from spoilt bread in Gwagwalada were not significantly different at P= 0.05 level of significance. The study demonstrated that Aspergillus flavus was able to produce extracellular protease enzymes important in the decomposition of protein materials.

Project Overview

1.0 INTRODUCTION1.1 Background of the studyProtease is the most important industrial enzyme of interest accounting for about 60% of the total enzyme market in the world and account for approximately 40% of the total worldwide enzyme sale (Godfrey and West, 1996; Chouyyok et al., 2005). They are generally used in detergents (Barindra et al., 2006), food industries, leather, meat processing, cheese making, silver recovery from photographic film, production of digestive and certain medical treatments of inflammation and virulent wounds (Rao et al., 1998; Paranthaman et al., 2009). They also have medical and pharmaceutical applications.Microbial proteases are degradative enzymes which catalyze the total hydrolysis of proteins (Raju et al., 1994; Haq et al., 2006). The molecular weight of proteases ranges from 18 - 90 kDa (Sidney and Lester, 1972). These enzymes are found in a wide diversity of sources such as plants, animals and microorganisms but they are mainly produced by bacteria and fungi. Microbial proteases are predominantly extracellular and can be secreted in the fermentation medium.In the production of protease, it has been shown to be inducible and was affected by the nature of the substrate used in fermentation. Therefore, the choice of an appropriate inducing substrate is of great importance. Different carbon sources such as wheat bran, rice straw, rice bran, cotton and bagasse have been studied for the induction and biosynthesis of protease. However, wheat bran is a superior carbon source for the production of protease by Aspergillus flavus. So the further studies were carried out by using wheat bran as carbon source.The use of agro-industrial residues as the basis for cultivation media is a matter of great interest, aiming to decrease the costs of enzyme production and meeting the increase in awareness on energy conservation and recycling (Singh et al., 2009). Major impediments to the exploitation of commercial enzymes are their yield, stability, specificity and the cost of production. New enzymes for use in commercial applications with desirable biochemical and physicochemical characteristics and low production cost have been focus of much research (Kabli, 2007). Solid state fermentation (SSF) was chosen for the present research because it has been reported to be of more grated productivity than that of submerged fermentation (Ghildyal et al., 1985; Hesseltine, 1972). Economically, SSF offers many advantages including superior volumetric productivity, use of simpler machinery, use of inexpensive substrates, simpler downstream processing, and lower energy requirements when compared with submerged fermentation (Paranthaman et al., 2009).1.2 Aim of the studyThe aim of this study was to produce protease from Aspergillus flavus using wheat bran as a substrate under Solid State Fermentation.1.3 Objectives of the studyThe objectives of the study include:-To isolate Aspergillus flavus from spoilt bread in Gwagwalada.-To determine the frequencies of occurrence of the isolated Aspergillus flavus from spoilt bread using simple percentages.-To determinethe proteolytic potential of the isolated fungi using basal medium.-To determine the quantity of the protease enzyme produced by the isolated fungi using spectrophotometer.

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