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FARWA FIAZ
13091514-057
BS 6th (B)
TOPIC
“ION EXCHANGE CHROMATOGRAPHY”
• INTRODUCTION:
• It is a process that separates ions and polar molecules
based on their affinity to the ion exchanger.
• An ion exchanger is something that is supposed to attract
positive or negative charges.(charged resin in this case)
• This process is used for proteins, small nucleotides, and
amino acids.
• It is mostly used in protein purification and water
analysis.
• TYPES
• Following are the two type of ion exchange
chromatography:
1. Cation exchange chromatography
• In this type positively charged molecules are
attracted to a negatively charged ion
exchanger
• Commonly used cation exchanger are sulfate
derivatives, S-resin and
carboxylate derived ions
2. Anion exchange chromatography
In this type negatively charged molecules are
attracted to a positively charged solid
support(ION EXCHANGER)
Commonly used anion exchange resins are
Q-resin and DEAE resin.
TWO PHASES
• The stationary phase is a resin on which usually
organic coating provides a charged surface. It is
fixed and immobilized.
• The mobile phase may be a liquid or gas, that
moves the sample components through a region
containing the solid or liquid stationary phase.
Base solutions and salt solutions can be used as
the mobile phase.
PRINCIPLE:
1.Equilibration
• At this stage whole surface of charged resin is
equally surrounded by salt molecules or buffer
2.Sample application and Adsorption
• The impure sample for example of protein is
applied from the top of the tube it may contain
+ve,-ve or neutral groups
• Molecules having opposite charge will bound
charged resin. This binding will depend on the
suitable PH.
• 3. ELUTION
• By increasing the ionic strength or concentration of
buffer,it will displace or release all the bound protein
charges and unbound impurities and move them down
the tube to elute them out,charged protein molecules
will take longer time to unbound from charged resin so
it can be purified and isolated according to this
property. This process is called elusion.
• 4.Regeneration
• Buffer ions removes protein molecules still bound to
ion exchanger. This ensures that stationary phase is
available for the next run.
urple
• At the very first step sample is shown in
purple color
• Then buffer is applied which wash out all the
bound and unbound sample materials
• Liquid in blue color( last test tube) will be
purified desired sample

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Ion Exchange Chromatography

  • 3. • INTRODUCTION: • It is a process that separates ions and polar molecules based on their affinity to the ion exchanger. • An ion exchanger is something that is supposed to attract positive or negative charges.(charged resin in this case) • This process is used for proteins, small nucleotides, and amino acids. • It is mostly used in protein purification and water analysis.
  • 4. • TYPES • Following are the two type of ion exchange chromatography: 1. Cation exchange chromatography • In this type positively charged molecules are attracted to a negatively charged ion exchanger • Commonly used cation exchanger are sulfate derivatives, S-resin and carboxylate derived ions
  • 5. 2. Anion exchange chromatography In this type negatively charged molecules are attracted to a positively charged solid support(ION EXCHANGER) Commonly used anion exchange resins are Q-resin and DEAE resin.
  • 6. TWO PHASES • The stationary phase is a resin on which usually organic coating provides a charged surface. It is fixed and immobilized. • The mobile phase may be a liquid or gas, that moves the sample components through a region containing the solid or liquid stationary phase. Base solutions and salt solutions can be used as the mobile phase.
  • 7. PRINCIPLE: 1.Equilibration • At this stage whole surface of charged resin is equally surrounded by salt molecules or buffer 2.Sample application and Adsorption • The impure sample for example of protein is applied from the top of the tube it may contain +ve,-ve or neutral groups • Molecules having opposite charge will bound charged resin. This binding will depend on the suitable PH.
  • 8. • 3. ELUTION • By increasing the ionic strength or concentration of buffer,it will displace or release all the bound protein charges and unbound impurities and move them down the tube to elute them out,charged protein molecules will take longer time to unbound from charged resin so it can be purified and isolated according to this property. This process is called elusion. • 4.Regeneration • Buffer ions removes protein molecules still bound to ion exchanger. This ensures that stationary phase is available for the next run.
  • 9. urple • At the very first step sample is shown in purple color • Then buffer is applied which wash out all the bound and unbound sample materials • Liquid in blue color( last test tube) will be purified desired sample