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1.High Performance Thin
Layer Chromatography
(HPTLC).
2.Recent development led
to the improvements in
various operations
involved.
3.Difference b/w TLC &
HPTLC – practical
technique than of the
physical phenomenon
(partition, adsorption)
on which separation is
Difference
TLC
Stationary
phase –
thin layer
of sorbent
(cellulose
powder /
silica gel)
Coating on
an inert,
rigid glass
plate foil –
separation
on flat with
two
dimensiona
l surface
HPTLC
Improved
separation
technique,
high
resolutions
& improved
quantitative
analysis
• Similar approach & same physical
properties of TLC.
• Principle of separation – adsorption.
• Mobile phase flows through b/c of
capillary action.
• Components move according to their
affinities towards adsorbent.
• Components – separated on
chromatographic plate.
Components - Greater
affinity towards
stationary phase travels
slower
Components - Lesser
affinity towards
stationary phase travels
faster
High concentrated
solution, as less
amount of sample
– applied.
Normal phase –
silica gel is pre -
coated
Reversed phase –
polar solvents are
used for dissolving
the sample.
Plates solvents –
non polar of
volatile type.
Layer – pre-
coated silica gel :
adsorbent.
Plates – similar as
TLC. Particle size
– very fine
particles.
Plates : 4-5mm
silica gel to form
200mm layer
Fine particles –
greater resolution
& sensitivity.
TLC : 5 – 20mm
HPTLC : 4 – 8mm
(particle size)
Plates
Pre - washing
Remove water
Volatile impurities
Cleaned by methanol
conditioning
Pre – washed
plates placed in
oven at 120c for 15
– 20 minutes
(conditioning)
Size not >1mm diameter
Self – loading capillary for
small volume of samples
Surface using platinum –
iridium tubing fused into end
of a length of glass tubing
 Low polarity of mobile phase – no need for
saturation.
 High polarity of mobile phase – saturation is
needed.
 Solution by trial & error where chemical
properties of solute & solvent solubility of analytic
adsorbent layer are considered.
 Linear development method.
 plate – vertically. placed in solvent system in a
suitable container.
 solvent – fed by capillary action &
chromatogram – from both the sides.
Chromatographic
development -
Methods
Circular
development
Anti – circular
device
Multiple
development
 Immediately after the
development is
completed, the plates
are removed from the
chamber and dried to
remove the frees of
mobile phase.
 Detection - known by
iodine vapor in iodine
chamber.
HPTLC – supplies with computer &
data recording & storing devices.
Development – scanned at selected UV
wavelength by instruments & detected
spots - peaks
Scanner – converts bond into peak &
peak heights / area related to
concentration of substance on the
spot.
Peak heights & area under spot –
measured by instrument & recorded as
% on the printer.
FEATUR
ES
Quality of
adsorbed
layer
Methods of
sample
application
Sample into
adsorbent
layer
Scanning
densitometer
s
• Pure silica gel with
narrow particle size.
• Diameter : 3-5µm.
• Chemically bonded
layers as reverse phase
plates.
• Layers – improved
adsorbents of 5000
plates.
• Difficult separation in
shorter time than TLC
1. Quality of
adsorbed
layer
• Lower sample capacity
& so the layer is
reduced.
• Sample volume : 100 –
200 cm gives 1mm
diameter.
• After plate
development – 10
times better detection
limits.
• Advantage – compact
starting spots –
increased no. of
samples.
2. Methods of
sample
application
• Critical process.
• Capillary volume :
100/200 nL – sealed into
glass support capillary –
convenient spotting
device in quantitative
measurements.
• Capillary tip – polished
for smooth planar surface
of small area (0.05mm)
when used as mechanical
applicator minimizes
damage to surface of
plate.
3. Sample into
adsorbent layer
• Scan individual spot by
reflectance / absorption
of a light beam.
• Transmitted / reflected
radiation – photograph
on chromatogram
revealing dark / light
zones for separated
compounds.
4. Scanning
densitometers
Clinical purpose (analysis of
drugs in blood)
Environmental analysis
Separation of compounds
Quantitative analysis of volatile
compounds
Separation & quantitative analysis
of thermally stable compounds
HPTLC

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HPTLC

  • 1.
  • 2. 1.High Performance Thin Layer Chromatography (HPTLC). 2.Recent development led to the improvements in various operations involved. 3.Difference b/w TLC & HPTLC – practical technique than of the physical phenomenon (partition, adsorption) on which separation is
  • 3. Difference TLC Stationary phase – thin layer of sorbent (cellulose powder / silica gel) Coating on an inert, rigid glass plate foil – separation on flat with two dimensiona l surface HPTLC Improved separation technique, high resolutions & improved quantitative analysis
  • 4. • Similar approach & same physical properties of TLC. • Principle of separation – adsorption. • Mobile phase flows through b/c of capillary action. • Components move according to their affinities towards adsorbent. • Components – separated on chromatographic plate.
  • 5. Components - Greater affinity towards stationary phase travels slower Components - Lesser affinity towards stationary phase travels faster
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  • 7.
  • 8. High concentrated solution, as less amount of sample – applied. Normal phase – silica gel is pre - coated Reversed phase – polar solvents are used for dissolving the sample. Plates solvents – non polar of volatile type.
  • 9. Layer – pre- coated silica gel : adsorbent. Plates – similar as TLC. Particle size – very fine particles. Plates : 4-5mm silica gel to form 200mm layer Fine particles – greater resolution & sensitivity. TLC : 5 – 20mm HPTLC : 4 – 8mm (particle size)
  • 10. Plates Pre - washing Remove water Volatile impurities Cleaned by methanol conditioning Pre – washed plates placed in oven at 120c for 15 – 20 minutes (conditioning)
  • 11. Size not >1mm diameter Self – loading capillary for small volume of samples Surface using platinum – iridium tubing fused into end of a length of glass tubing
  • 12.  Low polarity of mobile phase – no need for saturation.  High polarity of mobile phase – saturation is needed.  Solution by trial & error where chemical properties of solute & solvent solubility of analytic adsorbent layer are considered.
  • 13.  Linear development method.  plate – vertically. placed in solvent system in a suitable container.  solvent – fed by capillary action & chromatogram – from both the sides. Chromatographic development - Methods Circular development Anti – circular device Multiple development
  • 14.  Immediately after the development is completed, the plates are removed from the chamber and dried to remove the frees of mobile phase.  Detection - known by iodine vapor in iodine chamber.
  • 15. HPTLC – supplies with computer & data recording & storing devices. Development – scanned at selected UV wavelength by instruments & detected spots - peaks Scanner – converts bond into peak & peak heights / area related to concentration of substance on the spot. Peak heights & area under spot – measured by instrument & recorded as % on the printer.
  • 16. FEATUR ES Quality of adsorbed layer Methods of sample application Sample into adsorbent layer Scanning densitometer s
  • 17. • Pure silica gel with narrow particle size. • Diameter : 3-5µm. • Chemically bonded layers as reverse phase plates. • Layers – improved adsorbents of 5000 plates. • Difficult separation in shorter time than TLC 1. Quality of adsorbed layer • Lower sample capacity & so the layer is reduced. • Sample volume : 100 – 200 cm gives 1mm diameter. • After plate development – 10 times better detection limits. • Advantage – compact starting spots – increased no. of samples. 2. Methods of sample application
  • 18. • Critical process. • Capillary volume : 100/200 nL – sealed into glass support capillary – convenient spotting device in quantitative measurements. • Capillary tip – polished for smooth planar surface of small area (0.05mm) when used as mechanical applicator minimizes damage to surface of plate. 3. Sample into adsorbent layer • Scan individual spot by reflectance / absorption of a light beam. • Transmitted / reflected radiation – photograph on chromatogram revealing dark / light zones for separated compounds. 4. Scanning densitometers
  • 19. Clinical purpose (analysis of drugs in blood) Environmental analysis Separation of compounds Quantitative analysis of volatile compounds Separation & quantitative analysis of thermally stable compounds