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Isolation, partial purification and characterization of α-amylase from bacillus alcalophilus

 

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 α-amylase
2.2 Sources of α-amylase
2.3 Enzyme Kinetics of α-amylase
2.4 Industrial Applications of α-amylase
2.5 Factors Affecting α-amylase Activity
2.6 Stability of α-amylase
2.7 Purification Techniques of α-amylase
2.8 Characterization Methods of α-amylase
2.9 Recent Advances in α-amylase Research
2.10 Comparative Analysis of α-amylase from Different Sources

Chapter THREE

3.1 Research Methodology Overview
3.2 Selection of Bacillus Alcalophilus Strain
3.3 Cultivation and Production of α-amylase
3.4 Extraction and Partial Purification Techniques
3.5 Enzyme Assays and Activity Measurement
3.6 Characterization of α-amylase
3.7 Protein Analysis Methods
3.8 Statistical Analysis of Data

Chapter FOUR

4.1 Analysis of α-amylase Production
4.2 Partial Purification Results
4.3 Enzyme Kinetics Data Interpretation
4.4 Characterization Findings
4.5 Comparison with Literature Values
4.6 Discussion on Enzyme Stability
4.7 Implications for Industrial Applications
4.8 Limitations and Future Research Directions

Chapter FIVE

5.1 Summary of Findings
5.2 Conclusions Drawn from the Study
5.3 Contributions to the Field
5.4 Recommendations for Further Research
5.5 Final Thoughts and Acknowledgments

Project Abstract

The aim of this study was to isolate, partially purify and characterize α-Amylase from Bacillus alcalophilus. The enzyme (α-amylase) was isolated from Bacillus alcalophilus using cassava as only carbon source. 20 g of soil sample were weighed out and dissolved in 40 ml of distilled water in a clean conical flask, mixed vigorously and heated at 60oC for 60 min in water bath and taken as the stock culture. From the stock preparation, ten folds serial dilution were carried out and the 10-4 to 10-6 dilutions were plated out in a media plate. Percentage ammonium sulphate saturation, ammonium sulphate precipitation and gel filtrations were carried out to partially purify α-amylase from Bacillus alcalophilus. The α-amylase was then characterised by studying the effect of pH, change in temperature, substrate concentration and metal ion on the enzyme`s activity. The specific activity of the crude enzyme was 160.26 U/mg proteins. After ammonium sulphate precipitation and gel filtration, the specific activity were found to be 88.9 and 285.9U/mg protein, respectively. The optimum pH was found to be 7.5 and 70°C respectively. The α-amylase activity was found to be enhanced by Ca2+, Mg2+, Mn2+and mCo2+, whereas Fe2+ was found to have inhibitory effect. The enzyme retained more than 80% of its activity at 60 min in the presence of Ca2+, Mg2+ , Mn2+and Co2+, and lost up to 90% of its activity in the presence of Fe2+. In this study, Ca2+ maintained more stability of the enzyme than all other metal ions. The Michaelis-Mentens constant (Km) and maximum velocity (Vmax) obtained from the Line Weaver Burk plot of initial velocity data of different substrate concentrations were 1.159 mg/mL and 16.24 μmol/min respectively. In conclusion, this study revealed the potentials Bacillus alcalophilus to serve as other source of α-amylase, especially for industrial purposes.

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