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Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 1
Affinity Chromatography
Mr. Sagar Kishor Savale
[Department of Pharmacy (Pharmaceutics)]
2015-016
avengersagar16@gmail.com
1. Introduction
1.1 Chromatography
• Applies the principles of the “fractional” separation procedures
• Non-instrumental analysis which partitions components between two phases usually a
mobile phase and a stationary phase, based on the difference in the components physical
properties
• Can separate complex mixtures composed of many very similar components.
• Chromatography is often coupled with analytical instruments to complete analysis.
• A single chromatographic analysis can isolate, identify , and quantitate multiple
components of mixtures
1.2 History of Chromatography
• 1903 – Tswett, a Russian botanist coined the term chromatography. He passed plant
tissue extracts through a chalk column to separate pigments by differential adsorption
chromatogrpahy
• 1915 R.M Willstatter, German Chemist win Nobel Prize for similar experiement
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 2
• 1922 L.S Palmer, American scientist used Tswett’s techniques on various natural
products
• 1931 Richard Kuhn used chromatography to separate isomers oh polyene pigments;
this is the first known acceptance of chromatographic methods
• 1938 Thin Layer chromatography by Russian scientist N.A Izamailov and M.S Shraiber
• 1941 Liquid-Liquid partition chromatography developed by Archer John, Porter Martin
and Richard Laurence Millington Synge
• 1944 Paper Chromatography one of the most important methods in the development of
biotechnology
• 1945 Gas Chromatography 1st
analytical gas-solid (adsorption) chromatography
developed by Fritz Prior
• 1950 Gas Liquid Chromatography by Martin and Anthony James; Martin won the
Nobel Prize in 1952
• 1966 HPLC named by Csaba Horvath, but didn’t become a popular method until 1970s
• 1950s Ion-Exchange chromatography declassified this technique
• 1970s Ion Chromatography was developed by Hamish Small and co-workers at the
Dow Chemical company
• 1930s Affinity Chromatography was developed for the study of enzymes and other
proteins
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 3
1.3 Principles of Chromatography
Chromatography is used when there is a difference in the retention times of different
components
1.4 Two types of phases
1) Stationary phase
2) Mobile phases
1.5 Properties of Chromatographic Properties
1) Immiscible stationary and mobile phases
2) An arrangement where a mixture is deposited at one end of the
Stationary phase
3) Flow of the mobile phase towards the other end of the stationary
Phase
4) Different rates of partitioning for each component
5) Means for visualizing the separation of each component
1.6 Techniques
1) Ion Exchange Chromatography (IEC) - separates biomolecules based on the their
net surface charge
2) Ion Chromatography (IC) - more general form of IEC allows separation of ions and
polar molecules based on the charge properties of the molecules
3) Affinity Chromatography (AC) - is the purification of a biomolecule with respect to
the specific binding of that biomolecule due to the chemical structure
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 4
4) Gas Chromatography (GC) - is a technique used to separate organic molecules that
are volatile
5) Gas-Liquid Chromatography (GLC)
1.7 Terminology
• Elution - washing of the mixture
• Eluent - additional solvents used for elution
• Effluent - exiting fluid stream
• Residence - time spent on column
• Stationary Phase - Column packaging material
• Mobile Phase - fluid carrying the mixture of analytes
2. History of Affinity Chromatography
 1930s, first developed by A.Wilhelm Tiselius-a swedish biochemist, won the Nobel
Prize in 1948
 Used to study enzymes and other proteins
 Relies on the affinity of various biochemical compounds with specific properties
2.1 Affinity Chromatography
• Affinity Chromatography is essentially a sample purification technique, used primarily
for biological molecules such as proteins.
• It is a method of separating a mixture of proteins or nucleic acids (molecules) by
specific interactions of those molecules with a component known as a ligand, which is
immobilized on a support. If a solution of, say, a mixture of proteins is passed over
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 5
(through) the column, one of the proteins binds to the ligand on the basis of specificity
and high affinity (they fit together like a lock and key).
• The other proteins in the solution wash through the column because they were not able
to bind to the ligand.
2.2 Principle
• Affinity chromatography is one of the most diverse and powerful chromatographic
methods for purification of a specific molecule or a group of molecules from complex
mixtures
• It is based on highly specific biological interactions between two molecules such as
interactions between enzyme and substrate, receptor and ligand, or antibody and
antigen.
• These interactions which are typically reversible are used for purification by placing
one of the interacting molecules referred to as affinity ligand onto a solid matrix to
create a stationary phase while a target molecule is in the mobile phase.
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 6
• Many of the commonly used ligands coupled to affinity matrices are now commercially
available and are ready to use.
2.3 Chromatographic Media
• A matrix in its use here is a substance, usually in bead form to which a specific ligand
is covalently bound.
• In order to for the matrix to be effective it must have certain characters:
• It must be insoluble in solvents and buffers employed in the process
• It must be chemically and mechanically stable...
• It must be easily coupled to a ligand or spacer arm onto which the ligand can be
attached.
• It must exhibit good flow properties and have a relatively large surface area for
attachment
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 7
2.4 Immobilized Ligand
• The ligand can be selected only after the nature of the macromolecule to be isolated is
known.
• When a hormone receptor protein is to be purified by affinity chromatography, the
hormone itself is an ideal candidate for the ligand.
• For antibody isolation, an antigen or hapten may be used as ligand.
• If an enzyme is to be purified, a substrate analog, inhibitor, cofactor, or effector may be
used as an immobilized ligand.
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 8
2.5 Attachment of Ligand to Matrix
• Several procedures have been developed for the covalent attachment of the ligand to
the stationary phase. All procedures for gel modification proceed in two separate
chemical steps:
• Activation of the functional groups on the matrix and
• Joining of the ligand to the functional group on the matrix.
• A wide variety of activated gels is now commercially available. The most widely
used are described in the following:
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 9
3. Specificity is based on three aspect of affinity
1) Matrix: for ligand attachment.
2) Spacer arm: used to bind ligand to matrix.
3) Ligand: molecule that binds reversibly to a specific target molecule(site of
interaction)
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 10
4. Examples
 Antigen Antibody
 Antibody Antigen
 Substrate Enzyme
 DNA Histon
 Hormone Binding Protein/Receptor
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 11
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 12
5. Used of Affinity Chromatography
 Purify and concentrate a substance from a mixture into a buffering solution
 Reduce the amount of a substance in a mixture
 Discern what biological compounds bind to a particular substance, such as drugs
 Purify and concentrate an enzyme solution
6. Advantages Of Affınıty Chromatography
1) Extremely high specificity
2) High degrees of purity can be obtained
3) The process is very reproducible
4) The binding sites of biological molecules can be simply investigated
7. Dısadvantages Of Affınıty Chromatography
1) Expensive ligands
2) Leakage of ligand
3) Degradation of the solid support
4) Limited lifetime
5) Non-specific adsorption
6) Relatively low productivity
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 13
8. Applications
1) It is used for isolation and purification of all biological macromolecule.
2) It is used to purify nucleic acid, antibodies, and enzymes. Etc
3) To notice which biological compounds bind to a particular substance.
4) To reduce an amount of substance in a mixture
5) Used in Genetic Engineering - nucleic acid purification
6) Production of Vaccines - antibody purification from blood serum
7) And Basic Metabolic Research - protein or enzyme purification from cell free
extracts
Department of Pharmacy (Pharmaceutics) | Sagar savale
SAGAR SAVALE 14
9. References
• Modern Experimental Biochemistry-Rodney F. Boyer
• Introductory Practical Biochemistry-S.K Swahney, Randhir Sing
• http://en.wikipedia.org/wiki/Affinity_chromatography
• www.apsu.edu/reedr/.../Affinity%20Chromatography%201.ppt
• www.rpi.edu/dept/chem-eng/WWW/faculty/.../Lecture%2001.pdf -
• www.chemistryinnovation.co.uk/.../Technology%20Area%20Affinity%20Chrom
atography.pdf
• Uhlén M (2008). “Affinity as a tool in life science.”Biotechniques 44 (5): 649–54.
doi:10.2144/000112803.PMID 18474040.
• bioWORLD, Concanavalin A - Specifically binds to mannosy and glucosyl
residues of polysaccharides and glycoproteins.
• GE Healthcare Life Sciences, Immobilized lectin.

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Affinity chromatography

  • 1. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 1 Affinity Chromatography Mr. Sagar Kishor Savale [Department of Pharmacy (Pharmaceutics)] 2015-016 avengersagar16@gmail.com 1. Introduction 1.1 Chromatography • Applies the principles of the “fractional” separation procedures • Non-instrumental analysis which partitions components between two phases usually a mobile phase and a stationary phase, based on the difference in the components physical properties • Can separate complex mixtures composed of many very similar components. • Chromatography is often coupled with analytical instruments to complete analysis. • A single chromatographic analysis can isolate, identify , and quantitate multiple components of mixtures 1.2 History of Chromatography • 1903 – Tswett, a Russian botanist coined the term chromatography. He passed plant tissue extracts through a chalk column to separate pigments by differential adsorption chromatogrpahy • 1915 R.M Willstatter, German Chemist win Nobel Prize for similar experiement
  • 2. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 2 • 1922 L.S Palmer, American scientist used Tswett’s techniques on various natural products • 1931 Richard Kuhn used chromatography to separate isomers oh polyene pigments; this is the first known acceptance of chromatographic methods • 1938 Thin Layer chromatography by Russian scientist N.A Izamailov and M.S Shraiber • 1941 Liquid-Liquid partition chromatography developed by Archer John, Porter Martin and Richard Laurence Millington Synge • 1944 Paper Chromatography one of the most important methods in the development of biotechnology • 1945 Gas Chromatography 1st analytical gas-solid (adsorption) chromatography developed by Fritz Prior • 1950 Gas Liquid Chromatography by Martin and Anthony James; Martin won the Nobel Prize in 1952 • 1966 HPLC named by Csaba Horvath, but didn’t become a popular method until 1970s • 1950s Ion-Exchange chromatography declassified this technique • 1970s Ion Chromatography was developed by Hamish Small and co-workers at the Dow Chemical company • 1930s Affinity Chromatography was developed for the study of enzymes and other proteins
  • 3. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 3 1.3 Principles of Chromatography Chromatography is used when there is a difference in the retention times of different components 1.4 Two types of phases 1) Stationary phase 2) Mobile phases 1.5 Properties of Chromatographic Properties 1) Immiscible stationary and mobile phases 2) An arrangement where a mixture is deposited at one end of the Stationary phase 3) Flow of the mobile phase towards the other end of the stationary Phase 4) Different rates of partitioning for each component 5) Means for visualizing the separation of each component 1.6 Techniques 1) Ion Exchange Chromatography (IEC) - separates biomolecules based on the their net surface charge 2) Ion Chromatography (IC) - more general form of IEC allows separation of ions and polar molecules based on the charge properties of the molecules 3) Affinity Chromatography (AC) - is the purification of a biomolecule with respect to the specific binding of that biomolecule due to the chemical structure
  • 4. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 4 4) Gas Chromatography (GC) - is a technique used to separate organic molecules that are volatile 5) Gas-Liquid Chromatography (GLC) 1.7 Terminology • Elution - washing of the mixture • Eluent - additional solvents used for elution • Effluent - exiting fluid stream • Residence - time spent on column • Stationary Phase - Column packaging material • Mobile Phase - fluid carrying the mixture of analytes 2. History of Affinity Chromatography  1930s, first developed by A.Wilhelm Tiselius-a swedish biochemist, won the Nobel Prize in 1948  Used to study enzymes and other proteins  Relies on the affinity of various biochemical compounds with specific properties 2.1 Affinity Chromatography • Affinity Chromatography is essentially a sample purification technique, used primarily for biological molecules such as proteins. • It is a method of separating a mixture of proteins or nucleic acids (molecules) by specific interactions of those molecules with a component known as a ligand, which is immobilized on a support. If a solution of, say, a mixture of proteins is passed over
  • 5. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 5 (through) the column, one of the proteins binds to the ligand on the basis of specificity and high affinity (they fit together like a lock and key). • The other proteins in the solution wash through the column because they were not able to bind to the ligand. 2.2 Principle • Affinity chromatography is one of the most diverse and powerful chromatographic methods for purification of a specific molecule or a group of molecules from complex mixtures • It is based on highly specific biological interactions between two molecules such as interactions between enzyme and substrate, receptor and ligand, or antibody and antigen. • These interactions which are typically reversible are used for purification by placing one of the interacting molecules referred to as affinity ligand onto a solid matrix to create a stationary phase while a target molecule is in the mobile phase.
  • 6. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 6 • Many of the commonly used ligands coupled to affinity matrices are now commercially available and are ready to use. 2.3 Chromatographic Media • A matrix in its use here is a substance, usually in bead form to which a specific ligand is covalently bound. • In order to for the matrix to be effective it must have certain characters: • It must be insoluble in solvents and buffers employed in the process • It must be chemically and mechanically stable... • It must be easily coupled to a ligand or spacer arm onto which the ligand can be attached. • It must exhibit good flow properties and have a relatively large surface area for attachment
  • 7. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 7 2.4 Immobilized Ligand • The ligand can be selected only after the nature of the macromolecule to be isolated is known. • When a hormone receptor protein is to be purified by affinity chromatography, the hormone itself is an ideal candidate for the ligand. • For antibody isolation, an antigen or hapten may be used as ligand. • If an enzyme is to be purified, a substrate analog, inhibitor, cofactor, or effector may be used as an immobilized ligand.
  • 8. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 8 2.5 Attachment of Ligand to Matrix • Several procedures have been developed for the covalent attachment of the ligand to the stationary phase. All procedures for gel modification proceed in two separate chemical steps: • Activation of the functional groups on the matrix and • Joining of the ligand to the functional group on the matrix. • A wide variety of activated gels is now commercially available. The most widely used are described in the following:
  • 9. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 9 3. Specificity is based on three aspect of affinity 1) Matrix: for ligand attachment. 2) Spacer arm: used to bind ligand to matrix. 3) Ligand: molecule that binds reversibly to a specific target molecule(site of interaction)
  • 10. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 10 4. Examples  Antigen Antibody  Antibody Antigen  Substrate Enzyme  DNA Histon  Hormone Binding Protein/Receptor
  • 11. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 11
  • 12. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 12 5. Used of Affinity Chromatography  Purify and concentrate a substance from a mixture into a buffering solution  Reduce the amount of a substance in a mixture  Discern what biological compounds bind to a particular substance, such as drugs  Purify and concentrate an enzyme solution 6. Advantages Of Affınıty Chromatography 1) Extremely high specificity 2) High degrees of purity can be obtained 3) The process is very reproducible 4) The binding sites of biological molecules can be simply investigated 7. Dısadvantages Of Affınıty Chromatography 1) Expensive ligands 2) Leakage of ligand 3) Degradation of the solid support 4) Limited lifetime 5) Non-specific adsorption 6) Relatively low productivity
  • 13. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 13 8. Applications 1) It is used for isolation and purification of all biological macromolecule. 2) It is used to purify nucleic acid, antibodies, and enzymes. Etc 3) To notice which biological compounds bind to a particular substance. 4) To reduce an amount of substance in a mixture 5) Used in Genetic Engineering - nucleic acid purification 6) Production of Vaccines - antibody purification from blood serum 7) And Basic Metabolic Research - protein or enzyme purification from cell free extracts
  • 14. Department of Pharmacy (Pharmaceutics) | Sagar savale SAGAR SAVALE 14 9. References • Modern Experimental Biochemistry-Rodney F. Boyer • Introductory Practical Biochemistry-S.K Swahney, Randhir Sing • http://en.wikipedia.org/wiki/Affinity_chromatography • www.apsu.edu/reedr/.../Affinity%20Chromatography%201.ppt • www.rpi.edu/dept/chem-eng/WWW/faculty/.../Lecture%2001.pdf - • www.chemistryinnovation.co.uk/.../Technology%20Area%20Affinity%20Chrom atography.pdf • Uhlén M (2008). “Affinity as a tool in life science.”Biotechniques 44 (5): 649–54. doi:10.2144/000112803.PMID 18474040. • bioWORLD, Concanavalin A - Specifically binds to mannosy and glucosyl residues of polysaccharides and glycoproteins. • GE Healthcare Life Sciences, Immobilized lectin.