Types chrom

Khalid Hussain
Khalid HussainProfessor um University of the Punjab
Types of Chromatography
Classification of chromatography
•   According to separation mode:

    a) Adsorption chromatography
    b) Partition chromatography
    c) Ion-exchange chromatography
    d) Size exclusion chromatography
    e) Affinity chromatography
Classification of chrom. (cont.)
• According to mobile phase:
  a) Gas Chromatography
       i- Gas solid chromatography
     ii- Gas liquid chromatography
  b) Liquid chromatography
       i- Paper chromatography
     ii- Thin-layer chromatography
    iii- Column chromatography
Classification of chrom. (cont.)

• According to form of stationary phase
  a) Planar chromatography
      i- Paper chromatography
     ii- Thin-layer chromatography
  b) Column chromatography
      i- Gas chromatography
     ii- Liquid chromatography (LC/HPLC)
LIQUID-COLUMN CHROMATOGRAPHY
 A sample mixture is passed through a column
 packed with solid particles which may or may not be
 coated with another liquid.
 With the proper solvents, packing conditions, some
 components in the sample travel through the column
 more slowly than others resulting in the desired
 separation.
Types chrom
FOUR BASIC LIQUID CHROMATOGRAPHY

The basic liquid chromatography modes are
  named according to the mechanism involved:

1. Liquid/Solid Chromatography (adsorption chromatography)
   A. Normal Phase LSC
   B. Reverse Phase LSC
2. Liquid/Liquid Chromatography (partition chromatography)
   A. Normal Phase LLC
   B. Reverse Phase LLC
L C used for samples:
 containing large molecules/ionic
 containing substances with low vapor
  pressure (non-volatile substances)
 Substances thermally unstable
 Substances can’t be vaporized without
  decomposing
LIQUID SOLID CHROMATOGRAPHY


                                    Normal phase LS
                                    Reverse phase LS

                                            δ− δ+

                                       Si - O - H
               30 µ                    Silica Gel




 The separation mechanism in LSC is based on the
 competition of the components of the mixture sample
 for the active sites on an absorbent such as Silica Gel.
LIQUID SOLID CHROMATOGRAPHY


                         OH      HEXANE




           Si - OH




                               OH CH
                         CH3        3

                     CH3- C          C-CH3
                         CH3         CH3


                               CH3
Adsorption chromatography
   Stationery phase is solid and mobile phase is
    liquid
   Distribution between two phases (adsorption and
    desorption)
   Attractive forces (ionic, dipole-dipole, dipole
    induced dipole)
   Good adsorbent has large surface area and more
    active sites
   Equilibration occurs at: surface-solute, surface-
    solvent, solvent-solute
Adsorption isotherms
 An adsorption isotherm is a plot of the
  concentration or amount of analyte on a
  surface as a function of its concentration in
  the bulk phase.
 In liquid chromatography, the bulk phase is,
  of course, the mobile phase.
Adsorption isotherms
 Linear (k = Cs/Cm) = 1
 Convex (k = Cs/Cm1/n) where n >1
 Concave
Adsorbents
   Adsorbing power depends on
    1- chemical nature of the surface
    2- area available
    3- pretreatment
Commonly used adsorbents
 Alumina, Al2O3 ,(Aluminum oxide). It may
  be acidic, basic and neutral in nature.
  Available in various grades
 Silica gel (silicon dioxide). It is acidic in
  nature. Available in various grades.
 CaCO3
 Sucrose
 Starch
 cellulose
  Adsorbent should have uniform size and
  large surface area
 Weight of the adsorbent should be 20-50
  times more than the sample
Solvents & adsorbents
 Since adsorbents are polar, non-polar elute first.
  Usually, the elusion order is as: alkyl halids <
  saturated hydrocarbons< unsaturated
  hydrocarbons <ethers < esters < ketones < amines
  < alcohols < phenols < acids and bases. Polymeric
  compounds and salts often don’t elute
 The solvents in the order of polarity Hexane/Pet
  ether < CCl4 < toluene < dichloromethane <
  chloroform < diethyl ether < acetone < ethyl
  acetate < propanol < ethanol < methanol < acetic
  acid < water
Columns and packing
 Various sizes are available
 Wet method
 Dry method
 Sample loading and running the column
WATER-SOLUBLE VITAMINS

1.     Niacinamide                       2.    Pyridoxine
                                                      H 3C      N
          N
                                                         HO          CH 2OH
               CONH 2                                           CH 2OH

3.     Riboflavin
                CH 2OH
            HOCH
           HOCH               4. Thiamin
           HOCH
              CH 2
H 3C          N    N      O   H 3C       N    NH 2       S    CH 2CH 2OH
                         NH                                                Cl
H 3C          N                      N               N
                                              CH 2            CH 3
                     O
WATER-SOLUBLE VITAMINS
         2




             3

Inject                     4
     1

                                    Column: u Bondapak C18
                                    Solvent: MeOH
                                    Sample: Water-Soluble Vitamins
 0       5       10   15       20
LIQUID-LIQUID CHROMATOGRAPHY

                                 ODPN(oxydipropionylnitrile)


                                         Normal Phase LLC
                                         Reverse Phase LLC




                                  NCCH3 CH2 OCH2 CH2 CN(Normal)
                                  CH3 (CH2 ) 16 CH3 (Reverse)




The stationary solid surface is coated with a 2nd liquid (the
Stationary Phase) which is immiscible in the solvent (Mobile) phase.

Partitioning of the sample between 2 phases delays or retains some
components more than others to effect separation.
Advantages of Partition
            chromatography
   – Advantage over adsorption chromatography
 More reproducible and predictable
 Distribution coefficient is constant over a much
  greater range of concentration yielding sharper and
  symmetrical peaks
 It is also of two types
  1-Normal phase
  2-Reversed phase
Supports for stationary phase
 Silica gel
 Kieselguhr/Celite
 Cellulose
steps
 Sample preparation
 Sample loading
 Elution
 Detection: chemical methods; diverse types
  of detectors can be used
ION-EXCHANGE CHROMATOGRAPHY




                                               -     +
                                            SO3 Na




Separation is based on the competition of different ionic
compounds of the sample for the active sites on the ion-
exchange resin (column-packing).
Ion exchange chromatography
 A process where ions held by solid matrix
  are exchanged for counter ions in the
  solution
 Synthetic ion exchange resins are used for
  water purification and separation of ions
MECHANISM OF ION-EXCHANGE
CHROMATOGRAPHY OF AMINO ACIDS


                                                         pH2

                   -            +             +
             SO3        Na          H3N
                                                  COOH


  Ion-exchange Resin




                   -                      +
             SO3                    H3N
                                                     -
                                                  COO    pH4.5
                            +
                       Na
Chromatography of Amino Acids
    Stationary Phase                                                                           Mobile Phase
                                                    +
                                            H3N
                        -
               SO3 Na+
                                                                COOH
                                            +
                                        Na
                                                                         OH
                                    -                   +
                    SO3                         H3 N
                                                                COOH
   Exchange Resin

                    -
              SO3 H3N+
                                                COOH
                                                                                                   pH3.5
                                                                OH
                                -
                    SO3                         +
                                        H3 N
                                        +                       -             +      -
                            Na                      COO                   H       OH = H 2 O

                            +
                    Na

                     -
               SO3                  H3 N
                                            +
                                                            -        +        -
                                                COO              H        OH = H 2 O
                                -
                    SO3Na+

                                                                                                  pH4.5
Ions exchange resins
 Consist of three dimensional polymeric
  chains, cross linked by short chains, which
  carry ionisable functional groups.
 Based on ions these are of two types
    – Cation exchangers (weak or strong)
    – Anion exchangers (weak or strong)
Formation of resin
 Styrene  and divinylbenzene
 The number of cross linkers
  determine by the ratio of Styrene :
  divinylbenzene
 Increasing cross linkers increases
  the rigidity and reduces swelling
Ion-exchange chromatography can be used to
perform preparative separation of amino acids




Negatively charged resin binds selectively to
positively charged amino acids
Behavior of resin
 Important properties which determine
  behavior of resin are:
1- size of particles
2- degree of cross linking
3- nature of functional groups
4- number of functional groups
Theoretical principles
 Ion exchange equilibrium
 distribution coefficient (KD) indicates affinity of
  the resin for ions relative to hydrogen
 Generally, if KD is large, resin will incline to
  attract the ion
 Polyvalent ions are more attracted to the resin
  compared to mono-valent
   In groups where charges are same, the
    difference between KD is related to the size
    of the ion
Uses of ion exchange
          chromatography
 Ion separation
 Concentration of trace matters
 Separation of alkali and alkali earth metals
 Separation of amino acids, proteins,
  peptides, nucleic acid and nucleotides
 immunoglobulin
Steps
 Same to that of the others
 Detection: conduction measuring
Types chrom
Size exclusion chromatography
 Molecular gel chromatography, gel
  permeation, molecular sieving or molecular
  exclusion
 Stationary phase serves as molecular sieve
 Separate molecules based on size via
  sieving or filtration
 Adsorption and electrical charge play role
  in separation
Gels
 Open  three dimensional network formed by
  cross linking large ploymeric chains
 Polar groups absorb water and swell
 Have an exclusion limit i.e critical size of a
  molecule that can just penetrate the interior
Theoretical principles
 There are 2 kinds of solvent in the gel
  Vi = Volume within gel
  Vo = volume outside the beads of the gel
Large molecules will not be able to enter or penetrate the
  pores of the gel, hence their elution volume (Ve ) will be
                    Ve = Vo
Whereas, smaller molecules must be swept through Vo plus
  some additional volume which is a fraction of Vi
Ve = Vo + KDVi, where KD = distribution
   coefficient
KD = Average concentration of solute in gel/
   Average concentration of solute outside gel
KD value should be between 0 and 1
 If sieving action is the only mechanism of
   separation (KD=1) then
                     Ve = Vo + Vi
If K<1, It indicates solvent interacts with the gel
   (adsorption, hydrogen bonding)
Types of the gels
 Sephadex, dextran gel (classified by the
  amount of water regain)
 Biogel, polyacrylamide gel, inert series of
  gels, insoluble in water and common
  organic solvents
 Styragel rigid cross linked polystyrene gel
  useful at temperature > 150oC with organic
  solvents, it can be used under high pressure
Gel Filtration
Applications
   Desalting (removal of salts and small molecules
    from macromolecules)
   Concentrating (concentration of dilute solutions of
    macromolecules with MW> exclusion limit
   Fractionation (separation of mixture of closely
    related molecules having small difference in KD
    values namely proteins, peptides, nucleic acids,
    polysaccharides, enzymes and hormones)
Types of Chromatography
MOBILE PHASE                           LIQUID




                 Liquid-Liquid                       Liquid-Solid
FORMAT          Chromatography                     Chromatography
                  (Partition)                       (Adsorption)



STATIONARY                                               Solid
                       Liquid
PHASE




    Normal Phase                                Normal Phase     Reverse Phase
                           Reverse Phase


  Mobile Phase -           Mobile Phase -
        Nonpolar                Polar
  Stationary phase -       Stationary phase -
       Polar                    Nonpolar
Detectors

1.   Ultraviolet Detector

     200-400nm
     254 nm


2.   Reflective Index Detector

     Universal Detector
Types chrom
Affinity chromatography
 Separation where surface of inert phase has
  been modified to selectively bind
  compounds having specific functional
  group
 Binding force should be strong enough to
  effect separation but weak enough to get the
  compound when desired
Properties of Inert matrix
 Mechanically and chemically stable
 Large surface area
 Easily derivatized
 Good flow characteristics
 Examples (agarose, controlled pore glass,
  cellulose)
Spacer
 An arm to move active group away from the bead
  so that steric hindrances are at minimum
 Effectiveness depend on their
    – length
    – stability of the attachment to the bead
    – hydrophobic nature
    – presence of fixed charges and their concentration
   Affi-gel has spacer arm –O- (CH2)3 NH2
    [Oxypropylamine]
Affinity Chromatography
Affinity Chromatography
Selected ligands and their affinity
              compounds

Ligands           Affinity compounds

Diazo-NAD-        dehydrogenases

AMP analogues     NADP- binding proteins

Blue dextran      Yeast phosphofructokinase
2000
Methotrexate      Dihydrofolate reductase
B12               Transcobalamin I and II
Chromatographic techniques

 Classical LC
 TLC/ paper chromatography
 Modern LC
Classical chromatography
              technoques
   Glass or plastic columns
   Need skill
   Solvent flow (gravity, suction) and individual
    samples collected manually
   Detected using different detectors
   Detection and quantification achieved by manual
    analysis of fractions
   Results are recorded in the form of chromatogram
    (sample concentration vs fraction number)
Disadvantages
 Column packing procedure tedious
 Low column efficiency, long analysis time
 Technique depends on user
 Detection of solutes is labor intensive and
  takes a lot of time
Plane chromatography
 Plane surface rather than column
 2 dimensional
 Selective properties (use of two solvents)
 Include
    – Paper chromatography and
    – thin layer chromatography
Principles
 Principles are similar to column
 Successive equilibrations of the analyte
  between two phases
 Non ideal processes may cause zone
  spreading
 Degree of retention is Rf
    – Ratio between distance traveled by
     solute/distance traveled by solvent
Relation between Rf and K
   Rf = number of moles of solute in mobile
    phase/total moles in both phases
      = Cm Am/CmAm+ CsAs
Am and As are the cross sectional areas of two
 phases. By dividing Cm
Rf = Am/Am+AsCs/Cm = Am/Am+ KAs
Paper chromatography
 Mainly qualitative and semi quantiative
 Easy to perform
 Mechanisms
1- liquid liquid
2- adsorption
3- hydrogen bonding
4- ion exchange
Nature of the paper
 Highly purified cellulose
 Great affinity for water and polar solvents
 Paper may be impregnated with alumina,
  silica or ion exchange resin
Procedure
  Sample application
 Development
1- ascending
 Simple and popular
 Solvent flow through capillary action
 Slow development
 Slow rate enhances partition, separation
2- descending
 Flow is downward
 Paper folded U shape
 Solvent flow capillary and gravity
 Much faster
detection
   Visible
   Application of Reagents
   UV absorbance
   Florescence
   IR
   Radioactivity
   Chemical tests
   Bioautography
qualitative
   Based on Rf values
Semi-quantitative
 Extraction and spectroscopy
 densitometry
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Types chrom

  • 2. Classification of chromatography • According to separation mode: a) Adsorption chromatography b) Partition chromatography c) Ion-exchange chromatography d) Size exclusion chromatography e) Affinity chromatography
  • 3. Classification of chrom. (cont.) • According to mobile phase: a) Gas Chromatography i- Gas solid chromatography ii- Gas liquid chromatography b) Liquid chromatography i- Paper chromatography ii- Thin-layer chromatography iii- Column chromatography
  • 4. Classification of chrom. (cont.) • According to form of stationary phase a) Planar chromatography i- Paper chromatography ii- Thin-layer chromatography b) Column chromatography i- Gas chromatography ii- Liquid chromatography (LC/HPLC)
  • 5. LIQUID-COLUMN CHROMATOGRAPHY A sample mixture is passed through a column packed with solid particles which may or may not be coated with another liquid. With the proper solvents, packing conditions, some components in the sample travel through the column more slowly than others resulting in the desired separation.
  • 7. FOUR BASIC LIQUID CHROMATOGRAPHY The basic liquid chromatography modes are named according to the mechanism involved: 1. Liquid/Solid Chromatography (adsorption chromatography) A. Normal Phase LSC B. Reverse Phase LSC 2. Liquid/Liquid Chromatography (partition chromatography) A. Normal Phase LLC B. Reverse Phase LLC
  • 8. L C used for samples:  containing large molecules/ionic  containing substances with low vapor pressure (non-volatile substances)  Substances thermally unstable  Substances can’t be vaporized without decomposing
  • 9. LIQUID SOLID CHROMATOGRAPHY Normal phase LS Reverse phase LS δ− δ+ Si - O - H 30 µ Silica Gel The separation mechanism in LSC is based on the competition of the components of the mixture sample for the active sites on an absorbent such as Silica Gel.
  • 10. LIQUID SOLID CHROMATOGRAPHY OH HEXANE Si - OH OH CH CH3 3 CH3- C C-CH3 CH3 CH3 CH3
  • 11. Adsorption chromatography  Stationery phase is solid and mobile phase is liquid  Distribution between two phases (adsorption and desorption)  Attractive forces (ionic, dipole-dipole, dipole induced dipole)  Good adsorbent has large surface area and more active sites  Equilibration occurs at: surface-solute, surface- solvent, solvent-solute
  • 12. Adsorption isotherms  An adsorption isotherm is a plot of the concentration or amount of analyte on a surface as a function of its concentration in the bulk phase.  In liquid chromatography, the bulk phase is, of course, the mobile phase.
  • 13. Adsorption isotherms  Linear (k = Cs/Cm) = 1  Convex (k = Cs/Cm1/n) where n >1  Concave
  • 14. Adsorbents  Adsorbing power depends on 1- chemical nature of the surface 2- area available 3- pretreatment
  • 15. Commonly used adsorbents  Alumina, Al2O3 ,(Aluminum oxide). It may be acidic, basic and neutral in nature. Available in various grades  Silica gel (silicon dioxide). It is acidic in nature. Available in various grades.  CaCO3  Sucrose  Starch  cellulose
  • 16.  Adsorbent should have uniform size and large surface area  Weight of the adsorbent should be 20-50 times more than the sample
  • 17. Solvents & adsorbents  Since adsorbents are polar, non-polar elute first. Usually, the elusion order is as: alkyl halids < saturated hydrocarbons< unsaturated hydrocarbons <ethers < esters < ketones < amines < alcohols < phenols < acids and bases. Polymeric compounds and salts often don’t elute  The solvents in the order of polarity Hexane/Pet ether < CCl4 < toluene < dichloromethane < chloroform < diethyl ether < acetone < ethyl acetate < propanol < ethanol < methanol < acetic acid < water
  • 18. Columns and packing  Various sizes are available  Wet method  Dry method  Sample loading and running the column
  • 19. WATER-SOLUBLE VITAMINS 1. Niacinamide 2. Pyridoxine H 3C N N HO CH 2OH CONH 2 CH 2OH 3. Riboflavin CH 2OH HOCH HOCH 4. Thiamin HOCH CH 2 H 3C N N O H 3C N NH 2 S CH 2CH 2OH NH Cl H 3C N N N CH 2 CH 3 O
  • 20. WATER-SOLUBLE VITAMINS 2 3 Inject 4 1 Column: u Bondapak C18 Solvent: MeOH Sample: Water-Soluble Vitamins 0 5 10 15 20
  • 21. LIQUID-LIQUID CHROMATOGRAPHY ODPN(oxydipropionylnitrile) Normal Phase LLC Reverse Phase LLC NCCH3 CH2 OCH2 CH2 CN(Normal) CH3 (CH2 ) 16 CH3 (Reverse) The stationary solid surface is coated with a 2nd liquid (the Stationary Phase) which is immiscible in the solvent (Mobile) phase. Partitioning of the sample between 2 phases delays or retains some components more than others to effect separation.
  • 22. Advantages of Partition chromatography – Advantage over adsorption chromatography  More reproducible and predictable  Distribution coefficient is constant over a much greater range of concentration yielding sharper and symmetrical peaks  It is also of two types 1-Normal phase 2-Reversed phase
  • 23. Supports for stationary phase  Silica gel  Kieselguhr/Celite  Cellulose
  • 24. steps  Sample preparation  Sample loading  Elution  Detection: chemical methods; diverse types of detectors can be used
  • 25. ION-EXCHANGE CHROMATOGRAPHY - + SO3 Na Separation is based on the competition of different ionic compounds of the sample for the active sites on the ion- exchange resin (column-packing).
  • 26. Ion exchange chromatography  A process where ions held by solid matrix are exchanged for counter ions in the solution  Synthetic ion exchange resins are used for water purification and separation of ions
  • 27. MECHANISM OF ION-EXCHANGE CHROMATOGRAPHY OF AMINO ACIDS pH2 - + + SO3 Na H3N COOH Ion-exchange Resin - + SO3 H3N - COO pH4.5 + Na
  • 28. Chromatography of Amino Acids Stationary Phase Mobile Phase + H3N - SO3 Na+ COOH + Na OH - + SO3 H3 N COOH Exchange Resin - SO3 H3N+ COOH pH3.5 OH - SO3 + H3 N + - + - Na COO H OH = H 2 O + Na - SO3 H3 N + - + - COO H OH = H 2 O - SO3Na+ pH4.5
  • 29. Ions exchange resins  Consist of three dimensional polymeric chains, cross linked by short chains, which carry ionisable functional groups.  Based on ions these are of two types – Cation exchangers (weak or strong) – Anion exchangers (weak or strong)
  • 30. Formation of resin  Styrene and divinylbenzene  The number of cross linkers determine by the ratio of Styrene : divinylbenzene  Increasing cross linkers increases the rigidity and reduces swelling
  • 31. Ion-exchange chromatography can be used to perform preparative separation of amino acids Negatively charged resin binds selectively to positively charged amino acids
  • 32. Behavior of resin  Important properties which determine behavior of resin are: 1- size of particles 2- degree of cross linking 3- nature of functional groups 4- number of functional groups
  • 33. Theoretical principles  Ion exchange equilibrium  distribution coefficient (KD) indicates affinity of the resin for ions relative to hydrogen  Generally, if KD is large, resin will incline to attract the ion  Polyvalent ions are more attracted to the resin compared to mono-valent
  • 34. In groups where charges are same, the difference between KD is related to the size of the ion
  • 35. Uses of ion exchange chromatography  Ion separation  Concentration of trace matters  Separation of alkali and alkali earth metals  Separation of amino acids, proteins, peptides, nucleic acid and nucleotides  immunoglobulin
  • 36. Steps  Same to that of the others  Detection: conduction measuring
  • 38. Size exclusion chromatography  Molecular gel chromatography, gel permeation, molecular sieving or molecular exclusion  Stationary phase serves as molecular sieve  Separate molecules based on size via sieving or filtration  Adsorption and electrical charge play role in separation
  • 39. Gels  Open three dimensional network formed by cross linking large ploymeric chains  Polar groups absorb water and swell  Have an exclusion limit i.e critical size of a molecule that can just penetrate the interior
  • 40. Theoretical principles  There are 2 kinds of solvent in the gel Vi = Volume within gel Vo = volume outside the beads of the gel Large molecules will not be able to enter or penetrate the pores of the gel, hence their elution volume (Ve ) will be Ve = Vo Whereas, smaller molecules must be swept through Vo plus some additional volume which is a fraction of Vi
  • 41. Ve = Vo + KDVi, where KD = distribution coefficient KD = Average concentration of solute in gel/ Average concentration of solute outside gel KD value should be between 0 and 1 If sieving action is the only mechanism of separation (KD=1) then Ve = Vo + Vi If K<1, It indicates solvent interacts with the gel (adsorption, hydrogen bonding)
  • 42. Types of the gels  Sephadex, dextran gel (classified by the amount of water regain)  Biogel, polyacrylamide gel, inert series of gels, insoluble in water and common organic solvents  Styragel rigid cross linked polystyrene gel useful at temperature > 150oC with organic solvents, it can be used under high pressure
  • 44. Applications  Desalting (removal of salts and small molecules from macromolecules)  Concentrating (concentration of dilute solutions of macromolecules with MW> exclusion limit  Fractionation (separation of mixture of closely related molecules having small difference in KD values namely proteins, peptides, nucleic acids, polysaccharides, enzymes and hormones)
  • 45. Types of Chromatography MOBILE PHASE LIQUID Liquid-Liquid Liquid-Solid FORMAT Chromatography Chromatography (Partition) (Adsorption) STATIONARY Solid Liquid PHASE Normal Phase Normal Phase Reverse Phase Reverse Phase Mobile Phase - Mobile Phase - Nonpolar Polar Stationary phase - Stationary phase - Polar Nonpolar
  • 46. Detectors 1. Ultraviolet Detector 200-400nm 254 nm 2. Reflective Index Detector Universal Detector
  • 48. Affinity chromatography  Separation where surface of inert phase has been modified to selectively bind compounds having specific functional group  Binding force should be strong enough to effect separation but weak enough to get the compound when desired
  • 49. Properties of Inert matrix  Mechanically and chemically stable  Large surface area  Easily derivatized  Good flow characteristics  Examples (agarose, controlled pore glass, cellulose)
  • 50. Spacer  An arm to move active group away from the bead so that steric hindrances are at minimum  Effectiveness depend on their – length – stability of the attachment to the bead – hydrophobic nature – presence of fixed charges and their concentration  Affi-gel has spacer arm –O- (CH2)3 NH2 [Oxypropylamine]
  • 53. Selected ligands and their affinity compounds Ligands Affinity compounds Diazo-NAD- dehydrogenases AMP analogues NADP- binding proteins Blue dextran Yeast phosphofructokinase 2000 Methotrexate Dihydrofolate reductase B12 Transcobalamin I and II
  • 54. Chromatographic techniques  Classical LC  TLC/ paper chromatography  Modern LC
  • 55. Classical chromatography technoques  Glass or plastic columns  Need skill  Solvent flow (gravity, suction) and individual samples collected manually  Detected using different detectors  Detection and quantification achieved by manual analysis of fractions  Results are recorded in the form of chromatogram (sample concentration vs fraction number)
  • 56. Disadvantages  Column packing procedure tedious  Low column efficiency, long analysis time  Technique depends on user  Detection of solutes is labor intensive and takes a lot of time
  • 57. Plane chromatography  Plane surface rather than column  2 dimensional  Selective properties (use of two solvents)  Include – Paper chromatography and – thin layer chromatography
  • 58. Principles  Principles are similar to column  Successive equilibrations of the analyte between two phases  Non ideal processes may cause zone spreading  Degree of retention is Rf – Ratio between distance traveled by solute/distance traveled by solvent
  • 59. Relation between Rf and K  Rf = number of moles of solute in mobile phase/total moles in both phases = Cm Am/CmAm+ CsAs Am and As are the cross sectional areas of two phases. By dividing Cm Rf = Am/Am+AsCs/Cm = Am/Am+ KAs
  • 60. Paper chromatography  Mainly qualitative and semi quantiative  Easy to perform  Mechanisms 1- liquid liquid 2- adsorption 3- hydrogen bonding 4- ion exchange
  • 61. Nature of the paper  Highly purified cellulose  Great affinity for water and polar solvents  Paper may be impregnated with alumina, silica or ion exchange resin
  • 62. Procedure  Sample application  Development 1- ascending  Simple and popular  Solvent flow through capillary action  Slow development  Slow rate enhances partition, separation
  • 63. 2- descending  Flow is downward  Paper folded U shape  Solvent flow capillary and gravity  Much faster
  • 64. detection  Visible  Application of Reagents  UV absorbance  Florescence  IR  Radioactivity  Chemical tests  Bioautography
  • 65. qualitative  Based on Rf values Semi-quantitative  Extraction and spectroscopy  densitometry