Immobilized Enzyme Systems

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Presentation transcript:

Immobilized Enzyme Systems

THE ECONOMIC ARGUMENT FOR IMMOBILISATION Enzymes are expensive, they should be utilized in an efficient manner As catalytic molecules, enzymes are not directly used up. After the reaction the enzymes cannot be economically recovered for re-use and are generally wasted This enzyme residue remains to contaminate the product and its removal may involve extra purification costs Simple and economic methods must be used to separate the enzyme from the reaction product

This is known as IMMOBILISATION Separation of enzyme and product using a two- phase system; * One phase containing the enzyme * The other phase containing the product This is known as IMMOBILISATION

What is an Immobilized Enzyme?

Benefits of Immobilizing an Enzyme

METHODS OF IMMOBILISATION

Classification of Immobilization Methods for Enzymes

1. Entrapment The entrapment method of immobilization is based on the localization of an enzyme within the lattice of a polymer matrix or membrane. It is done in such a way as to retain protein while allowing penetration of substrate. It can be classified into lattice and micro capsule types.

Lattice-Type entrapment involves entrapping enzymes within the interstitial spaces of a cross-linked water-insoluble polymer. Some synthetic polymers such as polyarylamide, polyvinylalcohol, etc... and natural polymer (starch) have been used to immobilize enzymes using this technique. Microcapsule-Type entrapping involves enclosing the enzymes within semi permeable polymer membranes.

2. Membrane confinement Membrane confinement of enzymes may be achieved by a number of quite different methods, all of which depend for their utility on the semipermeable nature of the membrane. This must confine the enzyme whilst allowing free passage for the reaction products and, in most configurations, the substrates. Hollow fiber type of membrane can be used Although expensive, easy to use and convenient for any kinds of enzymes Liposome can be used for this purpose

3. Adsorption Simple method and high enzyme loading Incubating supporter with enzymes in an appropriate pH and ionic strength Driving force is hydrophobic intxn and salt bridge

4. Covalent Binding Mode Maximum 0.2 g enzyme/g matrix Very little leakage The most common methods in laboratory scale

Advantages and Disadvantages of Covalent Binding Method

Methods of Covalent Binding of Enzymes to Supports

Covalent Coupling

Cross-Linking

Advantages and Disadvantages

The most common reagent used for cross-linking is glutaraldehyde

Comparison between the methods

Immobilization enhances the stability of the enzyme

Kinetics of immobilized enzyme Km and Vmax are changed Specificity can be changed (trypsin hydrolyze pepsinogen into 15 fragments in solution, but into 10 as immobilized form)

Kinetics of immobilized enzyme in nonporous solid support

Kinetics of immobilized enzyme in nonporous solid support

Kinetics of immobilized enzyme in nonporous solid support

Kinetics of immobilized enzyme in porous matrix

Kinetics of immobilized enzyme in porous matrix

Kinetics of immobilized enzyme in porous matrix η (effectiveness factor) is defined as the rate with diffusion limitation versus the rate w/o diffusion limitation

Kinetics of immobilized enzyme in porous matrix

REFERENCES Michael L. Shuler and Fikret Kargı, Bioprocess Engineering: Basic Concepts (2 nd Edition),Prentice Hall, New York, 2002. 1. James E. Bailey and David F. Ollis, Biochemical Engineering Fundementals (2 nd Edition), McGraw-Hill, New York, 1986.

www.rpi.edu/dept/chem-eng/Biotech-Environ/IMMOB/Immob.htm - 3k - www.cheric.org/ippage/e/ipdata/2004/02/file/e200402-1001.pdf - www.cheric.org/ippage/e/ipdata/2004/05/file/e200405-1101.pdf - www.chem.metu.edu.tr/academic/toppare/resarea/enzym/enzym.htm - 27k - http://www.engr.usask.ca/classes/CHE/461/notes/lecture%2016/lecture%20notes-enzyme-immobilization%20of%20enzyme.ppt#348,5,Slide 5