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Purification by chromatography and formulation

HARINATHA REDDY ASWARTHA
HARINATHA REDDY ASWARTHA

Purification by chromatography and formulation

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Purification by Chromatography By Dr. Harinatha Reddy A ASSISTANT PROFESSOR
To download power point : Pay: 20 US $ or RS : 400 and send pay receipt to mail (biohari14@gmail.com). I will send power point to your mail id. Name: Harinatha Reddy Bank name: HDFC Account number: 50100203661752 IFC code: HDFC0000514 Bangalore Karnataka.
Introduction:  The biological products of fermentation (proteins, pharmaceuticals, diagnostic compounds and research materials) are very effectively purified by chromatography.  Chromatography usually consists of a stationary phase and mobile phase.
 The stationary phase is the porous solid matrix packed in a column (equilibrated with a suitable solvent) on to which the mixture of compounds to be separated is loaded.  The compounds are eluted by a mobile phase.
The different types of chromatography techniques used for separation of desired product(mainly proteins): Chromatography Principle Ion exchange chromatography Net charge Gel filtration chromatography Size and shape Affinity chromatography Net charge or Biological affinity and Molecular recognition
Ion-exchange chromatography: Ion-exchange chromatography depends on the ionic bonding of proteins to an inert matrix material.
Ion-exchange chromatography:  Two of the most commonly employed ion-exchange resins (inert matrix material) are:  Diethylaminoethyl cellulose: (+) (binds to negative charged molecules: Anion exchanger)(DEAE) and  Carboxymethyl cellulose (-) (CM): Cation exchanger.
Column pH: 11 buffer
 It involves the separation of molecules based on their surface charges.  Ion-exchangers are of two types (cation- exchangers which have negatively charged groups like carboxymethyl and sulfonate, and anion- exchangers with positively charged groups like diethylaminoethyl (DEAE).
 In ion-exchange chromatography, the pH of the medium is very crucial.  The ionic bound molecules can be eluted from the matrix by changing the pH of the elutant buffer.  Ion-exchange chromatography is useful for the purification of antibiotics, besides the purification of proteins.
 The resin is packed into a column, and the protein solution is allowed through the column in a buffer whose composition promotes the binding of some or all of the proteins to the resin.  Proteins are bound to the resin reversibly and can be displaced by increasing or changing the ionic strength (or pH) of the buffer. (which adds small ions to compete with the charged groups of the macromolecules for sites on the resin).  Proteins are eluted from the column in order from the least strongly bound to the most strongly bound.
Gel Filtration Chromatography or Size exclusion chromatography :
Gel Filtration Chromatography: Agarose or Sephadex G-150 beads are generally used in chromato grphy column
For example if a solution consists of two different proteins such as 75 kD and 120 kDa loaded on top of the colum.
 Gel filtration separates proteins (or nucleic acids) primarily on the basis of their effective size.  Like ion-exchange chromatography, the separation material consists of gel beads that are packed into a column through which the protein solution slowly passes.  The materials used in gel filtration are composed of cross-linked polysaccharides (agarose or Sephadex G-150 beads) of different porosity, which allow proteins to diffuse in and out of the beads.
 For example if a solution consists of three different proteins such as 120 kDa, 75 kDa and 25 kDa.  To purify 120 kDa protein form mixture, the sample pass through a column of Sephadex G-150 beads.  When the protein mixture passes through the column bed, the 120 kDa protein is unable to enter the beads and remains dissolved in the moving solvent phase.  The gel beads allows only the entry of proteins that are less than about 100 kDa size.
 As a result, the 120 kDa protein is eluted as soon as the preexisting solvent in the column (the bed volume) has dripped out.  In contrast, the other two proteins can diffuse into the interstices within the beads and are retarded in their passage through the column.  As more and more solvent moves through the column, these proteins move down its length and out the bottom, but they do so at different rates.  Among those proteins that enter the beads, smaller species are retarded to a greater extent than larger ones.  Consequently, the 120-kDa protein is eluted in a purified state, while the 75-kDa and 25 kDa protein remains in the column.
Affinity chromatography:
Affinity chromatography:
Affinity chromatography:  Affinity chromatography is based on an interaction of a protein with an immobilized ligand.  Such interactions including hydrogen bonding, ionic interaction, disulfide bridges, hydrophobic interaction,  The ligand can be a specific antibody, substrate, or an inhibitor or antigen or enzyme.  The protein bound to the ligand can be eluted by reducing their interaction. This can be achieved by changing the pH of the buffer.
Formulation: Formulation broadly refers to the maintenance of activity and stability of a biological products during storage and distribution.
Formulation:  For certain small molecules like (antibiotics, citric acid), formulation can be done by crystallization by adding salts.  The formulation of low molecular weight products can be achieved by concentrating them with removal of the water
 Proteins may be formulated in the form of solutions, or dry powders.  The sugars (sucrose, lactose), salts (sodium chloride, ammonium sulfate), glycerol used as stabilizers for protein formulation.  Vaccines are formulated by mixing with fluids (such as saline).
Drying (Formulation):  Drying is an essential component of product formulation.  It basically involves the transfer of heat to a wet product for removal of moisture.
 These two types of dryers are commercially available.  Spray drying:  Freeze-drying:
Spray drying:  Spray drying is a method of producing a dry powder from a liquid.  This method preferred method of drying of many thermally- sensitive materials such as foods and pharmaceuticals. stream of hot gas Spray dryer
 Spray drying is used for drying large volumes of liquids.  In spray drying, liquid containing the product are passed through a nozzle directing it over a stream of hot gas. (Liquid pumps in the form of droplets).  The water evaporates and the solid particles are left behind.  This method used for formation of milk powder.  Formulation of vitamins, enzymes, amino acids, antibiotics.
Freeze-drying:  Freeze-drying or lyophilization is the most preferred method for formulation of a wide-range of products.  Antibiotics, bacteria, viruses are formulated by using these process.  In this method, the product is rapidly frozen at a very low temperature (-70°C) and then dehydrated by vacuum.
• Under these conditions, the microbial cells are dehydrated and their metabolic activities are stopped; • as a result, the microbes go into dormant state and retain viability for years.
THANK Y OU:

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Purification by chromatography and formulation

  • 1. Purification by Chromatography By Dr. Harinatha Reddy A ASSISTANT PROFESSOR
  • 2. To download power point : Pay: 20 US $ or RS : 400 and send pay receipt to mail (biohari14@gmail.com). I will send power point to your mail id. Name: Harinatha Reddy Bank name: HDFC Account number: 50100203661752 IFC code: HDFC0000514 Bangalore Karnataka.
  • 3. Introduction:  The biological products of fermentation (proteins, pharmaceuticals, diagnostic compounds and research materials) are very effectively purified by chromatography.  Chromatography usually consists of a stationary phase and mobile phase.
  • 4.  The stationary phase is the porous solid matrix packed in a column (equilibrated with a suitable solvent) on to which the mixture of compounds to be separated is loaded.  The compounds are eluted by a mobile phase.
  • 5. The different types of chromatography techniques used for separation of desired product(mainly proteins): Chromatography Principle Ion exchange chromatography Net charge Gel filtration chromatography Size and shape Affinity chromatography Net charge or Biological affinity and Molecular recognition
  • 6. Ion-exchange chromatography: Ion-exchange chromatography depends on the ionic bonding of proteins to an inert matrix material.
  • 7. Ion-exchange chromatography:  Two of the most commonly employed ion-exchange resins (inert matrix material) are:  Diethylaminoethyl cellulose: (+) (binds to negative charged molecules: Anion exchanger)(DEAE) and  Carboxymethyl cellulose (-) (CM): Cation exchanger.
  • 9.  It involves the separation of molecules based on their surface charges.  Ion-exchangers are of two types (cation- exchangers which have negatively charged groups like carboxymethyl and sulfonate, and anion- exchangers with positively charged groups like diethylaminoethyl (DEAE).
  • 10.  In ion-exchange chromatography, the pH of the medium is very crucial.  The ionic bound molecules can be eluted from the matrix by changing the pH of the elutant buffer.  Ion-exchange chromatography is useful for the purification of antibiotics, besides the purification of proteins.
  • 11.  The resin is packed into a column, and the protein solution is allowed through the column in a buffer whose composition promotes the binding of some or all of the proteins to the resin.  Proteins are bound to the resin reversibly and can be displaced by increasing or changing the ionic strength (or pH) of the buffer. (which adds small ions to compete with the charged groups of the macromolecules for sites on the resin).  Proteins are eluted from the column in order from the least strongly bound to the most strongly bound.
  • 12. Gel Filtration Chromatography or Size exclusion chromatography :
  • 13. Gel Filtration Chromatography: Agarose or Sephadex G-150 beads are generally used in chromato grphy column
  • 14. For example if a solution consists of two different proteins such as 75 kD and 120 kDa loaded on top of the colum.
  • 15.  Gel filtration separates proteins (or nucleic acids) primarily on the basis of their effective size.  Like ion-exchange chromatography, the separation material consists of gel beads that are packed into a column through which the protein solution slowly passes.  The materials used in gel filtration are composed of cross-linked polysaccharides (agarose or Sephadex G-150 beads) of different porosity, which allow proteins to diffuse in and out of the beads.
  • 16.  For example if a solution consists of three different proteins such as 120 kDa, 75 kDa and 25 kDa.  To purify 120 kDa protein form mixture, the sample pass through a column of Sephadex G-150 beads.  When the protein mixture passes through the column bed, the 120 kDa protein is unable to enter the beads and remains dissolved in the moving solvent phase.  The gel beads allows only the entry of proteins that are less than about 100 kDa size.
  • 17.  As a result, the 120 kDa protein is eluted as soon as the preexisting solvent in the column (the bed volume) has dripped out.  In contrast, the other two proteins can diffuse into the interstices within the beads and are retarded in their passage through the column.  As more and more solvent moves through the column, these proteins move down its length and out the bottom, but they do so at different rates.  Among those proteins that enter the beads, smaller species are retarded to a greater extent than larger ones.  Consequently, the 120-kDa protein is eluted in a purified state, while the 75-kDa and 25 kDa protein remains in the column.
  • 20. Affinity chromatography:  Affinity chromatography is based on an interaction of a protein with an immobilized ligand.  Such interactions including hydrogen bonding, ionic interaction, disulfide bridges, hydrophobic interaction,  The ligand can be a specific antibody, substrate, or an inhibitor or antigen or enzyme.  The protein bound to the ligand can be eluted by reducing their interaction. This can be achieved by changing the pH of the buffer.
  • 21. Formulation: Formulation broadly refers to the maintenance of activity and stability of a biological products during storage and distribution.
  • 22. Formulation:  For certain small molecules like (antibiotics, citric acid), formulation can be done by crystallization by adding salts.  The formulation of low molecular weight products can be achieved by concentrating them with removal of the water
  • 23.  Proteins may be formulated in the form of solutions, or dry powders.  The sugars (sucrose, lactose), salts (sodium chloride, ammonium sulfate), glycerol used as stabilizers for protein formulation.  Vaccines are formulated by mixing with fluids (such as saline).
  • 24. Drying (Formulation):  Drying is an essential component of product formulation.  It basically involves the transfer of heat to a wet product for removal of moisture.
  • 25.  These two types of dryers are commercially available.  Spray drying:  Freeze-drying:
  • 26. Spray drying:  Spray drying is a method of producing a dry powder from a liquid.  This method preferred method of drying of many thermally- sensitive materials such as foods and pharmaceuticals. stream of hot gas Spray dryer
  • 27.  Spray drying is used for drying large volumes of liquids.  In spray drying, liquid containing the product are passed through a nozzle directing it over a stream of hot gas. (Liquid pumps in the form of droplets).  The water evaporates and the solid particles are left behind.  This method used for formation of milk powder.  Formulation of vitamins, enzymes, amino acids, antibiotics.
  • 28. Freeze-drying:  Freeze-drying or lyophilization is the most preferred method for formulation of a wide-range of products.  Antibiotics, bacteria, viruses are formulated by using these process.  In this method, the product is rapidly frozen at a very low temperature (-70°C) and then dehydrated by vacuum.
  • 29. • Under these conditions, the microbial cells are dehydrated and their metabolic activities are stopped; • as a result, the microbes go into dormant state and retain viability for years.
  • 30.
  • 31.