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FLASH CHROMATOGRAPHY

 Also called as “medium pressure chromatography”

 “An air pressure driven hybrid of medium and short
  column chromatography optimized for rapid separation"

 Popularized by Clark Still of Columbia University

 An alternative to slow and often inefficient gravity-fed
  chromatography
Introduction..

 Differs from the conventional technique in 2 ways:

    Slightly smaller silica gel particles (250-400 mesh)
    are used, and
    Due to restricted flow of solvent caused by the small
    gel particles, pressurized gas (10-15 psi) used to
    drive the solvent through the column of stationary
    phase

  The net result is a rapid “over in a flash” and high
  resolution chromatography.
Column vs Flash Chromatography

       Traditional Column             Flash chromatography
        chromatography
                                  •   Pre-packed plastic
•   Glass columns with silica         cartridges
    gel
                                  •   Solvent is pumped
•    Separation is very slow          through the cartridge
    (typically many hours)
                                  •    Much quicker and more
•    End of the run, silica gel       reproducible
    must be
    removed, cleaned, dried       •   Remaining solvent
    and re-packed                     flushed out of the column
                                      using pressurized gas
•    Both time consuming
    and hazardous
Column chromatography   Flash chromatography
Modern flash chromatography systems are sold as pre-packed
plastic cartridges, and the solvent is pumped through the
cartridge.

Systems may also be linked with detectors and fraction
collectors providing automation.

The introduction of gradient pumps resulted in quicker
separations and less solvent usage.

Flash chromatography is not expected to provide the resolution
or reproducibility of HPLC; it is a technique that can quickly
improve the purity of samples to an acceptable level.
Selection of solvent system
Solvent system

  Compound should have TLC Rf of 0.15 to 0.20 in the solvent
   system

  Binary solvent system –
    Polarity can be adjusted
    Rate of elution can be determined
   Common solvents used :
       dichloromethane/hexane, ether/hexane, hexane/ethyl
        acetate, and dichloromethane/methanol
   High polarity of solvents increase the rate of elution of all
                           compounds.
Quantity of silica gel required..

 40-63 µm silica gel particles are used

 Amount depends on 2 factors :
   – Rf difference of the compounds to be separated
   – Amount of sample

 ↑ silica gel -↑ the length of time for chromatography

 For,
   – Easier separations, ratios closer to 30 : 1 are effective
   – Difficult separations, more silica gel is often required
Packing the column

 Glass column / plastic cartridges

 Has either a glass frit or a plug of cotton wool directly above the
  stopcock (To prevent the silica gel from escaping from the
  column through the stopcock)

 ~1/2 inches layer of clean sand above the plug of glass wool

 Make sure that surface is flat

 Pour in the silica gel using a funnel.(Do this step in hood)
Method

• A solvent is chosen which gives good separation and moves the
  desired component to Rf = 0.20 on analytical TLC

• A column of the appropriate diameter is selected and filled with 5-6
  in. of dry 40-63 µ silica gel

•   Column is solvated
    – The column is filled with solvent and pressure is used to rapidly
      push all the air from the silica gel

• The sample is applied and the column is refilled with solvent and
  eluted at a flow rate of 2 in./min

• Top of the column should never run dry
Procedure for Microscale Flash Column
                  Chromatography
 In microscale flash chromatography, the column need neither a
  pinchclamp or a stopcock at the bottom of the column to control
  the flow, nor does it need air-pressure connections at the top of
  the column.

 Instead, the solvent flows very slowly through the column by
  gravity until you apply air pressure at the top of the column with
  an ordinary Pasteur pipet bulb.
(1) Prepare the column.




1. Plug a Pasteur pipet with a small          Add dry silica gel adsorbent, 230-400
amount of cotton; use a wood applicator       mesh -- usually the jar is labeled "for
stick to tamp it down lightly.                flash chromatography." One way to fill
                                              the column is to invert it into the jar of
2. Take care that you do not use either
                                              silica gel and scoop it out . . .
too much cotton or pack it too tightly. You
just need enough to prevent the
adsorbent from leaking out.
. . . then tamp it down before scooping   Another way to fill the column is to pour the
more out                                  gel into the column using a 10 mL beaker.
(2) Pre-elute the column.
(3) Load the sample onto the silica gel column

Two different methods are used to load the column: the wet
method and the dry method:
Wet loading method
The sample to be purified (or separated into components) is dissolved in a small amount
of solvent, such as hexanes, acetone, or other solvent. This solution is loaded onto the
column.
Dry loading method
(4) Elute the column.
5) Elute the column with the second elution solvent.

If separating a mixture of one or more compounds, at this point
change the eluting solvent to a more polar system, Elution would
proceed as in step (4).


(6) Analyze the fractions.

If the fractions are colored, simply combine like-colored
fractions, although TLC before combination is usually advisable.

If the fractions are not colored, they are analyzed by TLC
(usually). Once the composition of each fraction is known, the
fractions containing the desired compound(s) are combined.
Advantages
• Large quantities of the sample can be separated (0.5-2g)

• Fast ( 1o to 15 minutes)

• Cost efficient

• Elaborate equipment and the purchase of expensive
  equipment is not necessary

• If high resolution is required, flash chromatography is
  carried out before HPLC to avoid contamination of the
  expensive plates
Applications

• Purification of various peptides, antibiotics

• Separation of closely related organic compounds

• Purification of closely related drug intermediates

• High speed fractionation of natural products –
  tocopherols, alkaloids, lignans, xanthones, stilbenes, flavonoids

• Drug discovery

• Agrochemistry

• Petrochemistry
Conclusion

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Flash chromatography

  • 1. FLASH CHROMATOGRAPHY  Also called as “medium pressure chromatography”  “An air pressure driven hybrid of medium and short column chromatography optimized for rapid separation"  Popularized by Clark Still of Columbia University  An alternative to slow and often inefficient gravity-fed chromatography
  • 2. Introduction..  Differs from the conventional technique in 2 ways:  Slightly smaller silica gel particles (250-400 mesh) are used, and  Due to restricted flow of solvent caused by the small gel particles, pressurized gas (10-15 psi) used to drive the solvent through the column of stationary phase The net result is a rapid “over in a flash” and high resolution chromatography.
  • 3. Column vs Flash Chromatography Traditional Column Flash chromatography chromatography • Pre-packed plastic • Glass columns with silica cartridges gel • Solvent is pumped • Separation is very slow through the cartridge (typically many hours) • Much quicker and more • End of the run, silica gel reproducible must be removed, cleaned, dried • Remaining solvent and re-packed flushed out of the column using pressurized gas • Both time consuming and hazardous
  • 4. Column chromatography Flash chromatography
  • 5.
  • 6.
  • 7. Modern flash chromatography systems are sold as pre-packed plastic cartridges, and the solvent is pumped through the cartridge. Systems may also be linked with detectors and fraction collectors providing automation. The introduction of gradient pumps resulted in quicker separations and less solvent usage. Flash chromatography is not expected to provide the resolution or reproducibility of HPLC; it is a technique that can quickly improve the purity of samples to an acceptable level.
  • 8. Selection of solvent system Solvent system  Compound should have TLC Rf of 0.15 to 0.20 in the solvent system  Binary solvent system –  Polarity can be adjusted  Rate of elution can be determined Common solvents used : dichloromethane/hexane, ether/hexane, hexane/ethyl acetate, and dichloromethane/methanol High polarity of solvents increase the rate of elution of all compounds.
  • 9. Quantity of silica gel required..  40-63 µm silica gel particles are used  Amount depends on 2 factors : – Rf difference of the compounds to be separated – Amount of sample  ↑ silica gel -↑ the length of time for chromatography  For, – Easier separations, ratios closer to 30 : 1 are effective – Difficult separations, more silica gel is often required
  • 10. Packing the column  Glass column / plastic cartridges  Has either a glass frit or a plug of cotton wool directly above the stopcock (To prevent the silica gel from escaping from the column through the stopcock)  ~1/2 inches layer of clean sand above the plug of glass wool  Make sure that surface is flat  Pour in the silica gel using a funnel.(Do this step in hood)
  • 11. Method • A solvent is chosen which gives good separation and moves the desired component to Rf = 0.20 on analytical TLC • A column of the appropriate diameter is selected and filled with 5-6 in. of dry 40-63 µ silica gel • Column is solvated – The column is filled with solvent and pressure is used to rapidly push all the air from the silica gel • The sample is applied and the column is refilled with solvent and eluted at a flow rate of 2 in./min • Top of the column should never run dry
  • 12. Procedure for Microscale Flash Column Chromatography  In microscale flash chromatography, the column need neither a pinchclamp or a stopcock at the bottom of the column to control the flow, nor does it need air-pressure connections at the top of the column.  Instead, the solvent flows very slowly through the column by gravity until you apply air pressure at the top of the column with an ordinary Pasteur pipet bulb.
  • 13. (1) Prepare the column. 1. Plug a Pasteur pipet with a small Add dry silica gel adsorbent, 230-400 amount of cotton; use a wood applicator mesh -- usually the jar is labeled "for stick to tamp it down lightly. flash chromatography." One way to fill the column is to invert it into the jar of 2. Take care that you do not use either silica gel and scoop it out . . . too much cotton or pack it too tightly. You just need enough to prevent the adsorbent from leaking out.
  • 14. . . . then tamp it down before scooping Another way to fill the column is to pour the more out gel into the column using a 10 mL beaker.
  • 15. (2) Pre-elute the column.
  • 16. (3) Load the sample onto the silica gel column Two different methods are used to load the column: the wet method and the dry method: Wet loading method The sample to be purified (or separated into components) is dissolved in a small amount of solvent, such as hexanes, acetone, or other solvent. This solution is loaded onto the column.
  • 18. (4) Elute the column.
  • 19. 5) Elute the column with the second elution solvent. If separating a mixture of one or more compounds, at this point change the eluting solvent to a more polar system, Elution would proceed as in step (4). (6) Analyze the fractions. If the fractions are colored, simply combine like-colored fractions, although TLC before combination is usually advisable. If the fractions are not colored, they are analyzed by TLC (usually). Once the composition of each fraction is known, the fractions containing the desired compound(s) are combined.
  • 20. Advantages • Large quantities of the sample can be separated (0.5-2g) • Fast ( 1o to 15 minutes) • Cost efficient • Elaborate equipment and the purchase of expensive equipment is not necessary • If high resolution is required, flash chromatography is carried out before HPLC to avoid contamination of the expensive plates
  • 21. Applications • Purification of various peptides, antibiotics • Separation of closely related organic compounds • Purification of closely related drug intermediates • High speed fractionation of natural products – tocopherols, alkaloids, lignans, xanthones, stilbenes, flavonoids • Drug discovery • Agrochemistry • Petrochemistry