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Analytical Techniques in
Pharmacology
Capt Htet Wai Moe
04/03/17
Introduction
• From the stage of drug development to
marketing and post marketing, analytical
techniques play a great role
Common Analytical Techniques
• Titrimetry
• Chromatography
• Spectroscopy
• Capillary Electrophoresis
• Hyphenated techniques
Titrimetric techniques
Principle
• Addition of a reactant to a solution being
analyzed until some equivalence point is
reached
• Most familiar one is the acid-base titration
involving a color changing indicator
Fig. Titrimetry
Applications of Titrimetric techniques
• Provide standard pharmacopeial methods for
the assay of unformulated drugs and
excipients and some formulated drugs
• Used for standardization of raw materials and
intermediates used in drug synthesis
• Captopril, Albendazole, Gabapentin,
Sparfloxacin
Chromatography
Principle
• Separation technique used for separation of
mixture of low molecular weight compounds
based on their distribution in stationary phase
and mobile phase
Chromatographic techniques
• Thin Layer chromatography
• High performance thin layer chromatography
• High performance liquid chromatography
• Gas chromatography
Thin Layer chromatography (TLC)
Principle
• Chromatography technique used to separate
non-volatile mixtures
• Particles are separated based on partition or
adsorption
Thin Layer chromatography
• Performed on a sheet of glass, plastic , or
aluminum foil coated with a thin layer of
adsorbent material
• Adsorbent material – silica gel, aluminum
oxide or cellulose
• Adsorbent shows extreme selectivity toward
the substances being separated so as to the
dissimilarities in the rate of elution be large
Application of TLC
• Qualitative, quantitative, small scale and
preparative separation of amino acids,
steroids and nucleic acids
• Separation and isolation of large number of
inorganic compounds
• Various impurities of pharmaceuticals can be
identified and determined using TLC
High performance thin layer
chromatography (HPTLC)
Principle
• Enhanced form of thin layer chromatography
• Enhanced to automate the different steps, to
increase the resolution achieved, and to allow
more accurate quantitative measurements
• Automation is useful to overcome the
uncertainty in droplet size and position when
sample is applied to TLC plate by hand
Fig. HPTLC
Differences between TLC and HPTLC
Parameter TLC HPTLC
Chromatographic plate
used
Hand made/ pre-coated Pre-coated
Sorbent layer thickness 250 Âľm 100-200 Âľm
Particle size range 5-20 Âľm 4-8 Âľm
Application of sample
Manual/ Semi
automatic
Semi automatic/
Automatic
Sample volume 1-20 Âľl 0.2-5 Âľl
No. of samples/plate 15-20 40-50
Reproducibility of
results
Difficult Reproducible
High Performance Liquid
Chromatography (HPLC)
Principle
• Highly sensitive separation technique
• Sample and purified mobile phase are applied
to the column under high pressure
• Sample compounds are separated based on
adsorption, partition, ion exchange, molecular
exclusion or affinity principle
HPLC
• Relies on pumps to pass a pressurized liquid
solvent containing the sample mixture
through a column filled with a solid adsorbent
material
• Each component in the sample interacts
differently with the adsorbent material
HPLC
• Different flow rates for different components
lead to separation of components as they flow
out of the column
• Separate the complex mixture and recognize
the role of individual molecules
HPLC
Detectors in HPLC
• Choice of detectors is critical to guarantee that
all the components are detected
• Common types of detectors
– UV detector
– Photodiode array (PDA) detector
– Refractive index detector
– Fluorescence detector
UV detector
• Capable of monitoring several wavelengths
concurrently
• Can detect all the UV-absorbing components
UV detector
Photodiode array (PDA) detector
• Can sense a range of wavelengths
concurrently
• Wavelength range can be programmed and all
the compounds that absorb within this range
can be identified in a single analysis
Fig. Photodiode array detector
Refractive index detector
• Detector of choice to detect analytes with
restricted or no UV absorption such as
alcohols, sugars, carbohydrates, fatty acids,
and polymers
Fluorescence detector
• Most sensitive detectors
• 10-100 times higher than UV detector for
strong UV absorbing materials
Fluorescence detector
Applications of HPLC
• Manufacturing (e.g. during the production
process of pharmaceutical and biological
products)
• Legal (e.g. detecting performance
enhancement drugs in urine)
• Research (e.g. separating the components of a
complex biological sample)
• Medical (e.g. detecting Vitamin D levels in
blood serum)
Limitations of HPLC
• Price of columns and solvents
• Lack of long term reproducibility due to
proprietary nature of column packing
Gas Chromatography
Principle
• Used in analysis of the compounds that can be
vaporized without decomposition
• Testing the purity of a particular substance
• Separating the different components of
mixture
• Mobile phase is a carrier gas, usually an inert
gas such as helium or an unreactive gas such
as nitrogen
• Stationary phase is a microscopic layer of
liquid or polymer on an inert solid support
• Gaseous compounds being analyzed interact
with the walls of column
Gas Chromatography
Gas Chromatography
Applications of Gas Chromatography
• Assay of isotretinoin, cocaine and residual
solvents in betamethasone,
• Analysis of impurities of pharmaceuticals
• Identification of functional group of
compounds
Spectroscopy
• Analytical techniques used for quantification,
characterization and structural analysis of
macromolecules by measuring the absorption,
transmission, emission of radiation by the
molecules
Spectroscopic techniques
• UV-visible spectroscopy
• Mass spectrometry
• Near infrared spectroscopy
• Nuclear magnetic resonance spectroscopy
• Fluorimetry
• Phosphorimetry
UV-visible Spectroscopy
Category
Colorimetry Spectrophotometry
Beer’s Law
• Amount of light absorbed by a colored
solution is proportional to the concentration
of the solution
A Îą C
A = absorbance
C = concentration of the color in the solution
Lambert’s Law
• Amount of light absorbed by a colored
solution is proportional to the depth through
which the light passes in the solution
A Îą L
A = absorbance
L = depth through which light passes in the
solution
Colorimetry
• Quantification of colored compounds in
solution
Irradiating with visible light (400 – 700 nm)
Measuring the absorbance
Colorimetry
UV- Visible Spectrophotometry
• Quantification and characterization of
colorless compounds
Irradiating with UV (185-400 nm) or
visible light (400-700 nm)
Measuring the absorbance
UV-visible Spectrophotometry
Fig: Spectrophotometer
Applications of UV-visible
Spectroscopy
• To quantify protein, carbohydrates, Hb,
Chlorophyll
• To detect impurity in biological compounds
(Impurities are displayed as additional peaks
in spectrum)
Common Drugs analyzed by UV-
visible spectrophotometry
• Acetaminophen, Amlodipine, Ampicillin,
amoxycillin, Lisinopril, Flunarizine,
Carbenicillin, Diclofenac sodium, Diltiazem,
Nicorandil, Pantoprazole sodium, Zidovudine,
Verapamil
Mass Spectrometry
Principle
• Sample is ionized by bombarding it with high
energy electrons
• Some of the sample’s molecules to break into
charged fragments
• These ions are then separated according to
their mass-to-charge ratio
Mass Spectrometry (MS)
• Ions of the same mass-to-charge ratio will
undergo the same amount of deflection
• The ions are detected by electron multiplier
which can detect charged particles
• Results are displayed as spectra
Application of MS
• Elucidation of structure of organic and
biological molecules
• Determination of molecular mass of peptides,
proteins and oligonucleotides
• Identification of drugs abuse and metabolite
of drugs of abuse in blood, urine and saliva
Principle
• Uses light over the infrared range (700-15000
nm) of electromagnetic radiation spectrum
• The energy curve of an oscillating molecule is
affected by intramolecular interactions
• Vibrations around the equilibrium position
are non-symmetric and the spacings between
energy levels that the molecule can attain are
not identical
Near Infrared spectroscopy (NIRS)
• Easy preparation without any pretreatments
• Identification and qualification of raw
materials and intermediates
• Analysis of intact dosage forms
• Process monitoring and process control
Applications of (NIRS)
Near Infrared spectroscopy
Nuclear magnetic resonance
spectroscopy (NMR)
Principle
• The important property of nucleus is spinning
• Compound is subjected to external magnetic
field and radio wave
• Nucleus is promoted to higher magnetic
energy level and resonance occurs NMR
signal recorded as NMR peak gives
structural information about the compound
Applications of NMR
• To study the structure of antibiotics,
interleukin and nucleic acids
• To study drug metabolism
• For conformational analysis of
macromolecules
Fluorimetry
Principle
• Fluorescence is a phenomenon of emission of
radiation when the molecules are excited by
radiation at certain wavelength
• Fluorimetry measures the fluorescence
intensity at a particular wavelength with the
help of a filter fluorimeter
Fluorimetry
Fig. FLuorimeter
Applications of Fluorimetry
• High sensitive technique to identify the
presence and amount of specific molecules
• Quantitative analysis of various drugs in
dosage forms and biological fluids
Phosphorimetry
Principle
• Phosphorescence is also a phenomenon of
emission of radiation when the molecules are
excited by radiation at certain wavelength
• Difference from fluorimetry – emission of
radiation continues after light source is cut off
• Applications – Analysis of Quinolone,
Riboflavin, Anticancer drugs, Naproxen
Capillary Electrophoresis
Principle
• Separation of compounds that are capable of
acquiring electric charge in conduction
electrodes
• Based on difference in migration of charged
particle through a solution under the
influence of an external electrical field
Capillary Electrophoresis
• Solutes are perceived as peaks as they pass
through detector and the area of individual
peak is proportional to concentration
• Quicker time scale, requirement of only a
small amount up to Nano liter injection
volumes
• Applications – Separation of Atropine
sulphate, Codeine phosphate, Ketamine HCL,
Phenylephrine HCL
Fig. Capillary electrophoresis
Fig. Capillary electrophoresis
Hyphenated techniques
• Provides more information than could be
obtained by using the individual techniques in
isolation
• Time saving
• Additional information
Hyphenated techniques
• Hyphenated techniques combine
chromatographic and spectral methods to
exploit the advantages of both
• Chromatography produces pure or nearly pure
fractions of chemical components in a mixture
• Spectroscopy produces selective information
for identification using standards or library
spectra
• GC-MS
Gas chromatography–mass spectrometry
• LC-MS
Liquid chromatography–mass spectrometry
• LC-IR
Liquid chromatography–Infrared Spectroscopy
• LC-NMR
Liquid chromatography–Nuclear magnetic
resonance spectroscopy
• CE-MS
Capillary electrophoresis–mass spectrometry
Hyphenated techniques
GC-MS
• Compounds that are adequately volatile, small
and stable in high temperature in GC conditions
can be easily analyzed by GC-MS
• A carrier gas propels the sample down the
column
• GC separates the components of a mixture in
time
• MS detector provides information that aids in the
structural identification of each component
LC-MS
• Separated sample emerging from the column
can be identified on the basis of its mass
spectral data
• Combines chemical separating power of LC
with the ability of MS to selectively detect and
confirm molecular identity
LC-IR
• Coupling of LC and detection method infrared
spectrometry (IR)
• IR is useful spectroscopic technique for
identification of organic compounds
LC-NMR
• Analysis of complex mixtures of all types,
particularly the analysis of natural products
and drug-related metabolites in biofluids
• Reversed-phase columns are used in LC-NMR
CE-MS
• Almost all molecules can be separated using
this powerful method
• Separates species by applying voltage across
buffer-filled capillaries
• Generally used for separating ions that move
at different speeds when voltage is applied,
depending on their size and charge
References
• Julia C Drees, Alan H B Wu. Analytical
techniques. In: Michael L Bishop, editor.
Clinical chemistry. 5th Ed, Lippincott Williams
& Wilkins 2010; 130-165.
• Glen L Hortin, Bruce A Goldberger.
Chromatography and Extraction. In: Tietz
Textbook of Clinical Chemistry and Molecular
Diagnostics. 5th Ed, Elsevier 2012; 307-328.
THANK YOU!

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Analytical Techniques in Pharmacology

  • 2. Introduction • From the stage of drug development to marketing and post marketing, analytical techniques play a great role
  • 3. Common Analytical Techniques • Titrimetry • Chromatography • Spectroscopy • Capillary Electrophoresis • Hyphenated techniques
  • 4. Titrimetric techniques Principle • Addition of a reactant to a solution being analyzed until some equivalence point is reached • Most familiar one is the acid-base titration involving a color changing indicator
  • 6. Applications of Titrimetric techniques • Provide standard pharmacopeial methods for the assay of unformulated drugs and excipients and some formulated drugs • Used for standardization of raw materials and intermediates used in drug synthesis • Captopril, Albendazole, Gabapentin, Sparfloxacin
  • 7. Chromatography Principle • Separation technique used for separation of mixture of low molecular weight compounds based on their distribution in stationary phase and mobile phase
  • 8. Chromatographic techniques • Thin Layer chromatography • High performance thin layer chromatography • High performance liquid chromatography • Gas chromatography
  • 9. Thin Layer chromatography (TLC) Principle • Chromatography technique used to separate non-volatile mixtures • Particles are separated based on partition or adsorption
  • 10. Thin Layer chromatography • Performed on a sheet of glass, plastic , or aluminum foil coated with a thin layer of adsorbent material • Adsorbent material – silica gel, aluminum oxide or cellulose • Adsorbent shows extreme selectivity toward the substances being separated so as to the dissimilarities in the rate of elution be large
  • 11.
  • 12. Application of TLC • Qualitative, quantitative, small scale and preparative separation of amino acids, steroids and nucleic acids • Separation and isolation of large number of inorganic compounds • Various impurities of pharmaceuticals can be identified and determined using TLC
  • 13. High performance thin layer chromatography (HPTLC) Principle • Enhanced form of thin layer chromatography • Enhanced to automate the different steps, to increase the resolution achieved, and to allow more accurate quantitative measurements • Automation is useful to overcome the uncertainty in droplet size and position when sample is applied to TLC plate by hand
  • 15. Differences between TLC and HPTLC Parameter TLC HPTLC Chromatographic plate used Hand made/ pre-coated Pre-coated Sorbent layer thickness 250 Âľm 100-200 Âľm Particle size range 5-20 Âľm 4-8 Âľm Application of sample Manual/ Semi automatic Semi automatic/ Automatic Sample volume 1-20 Âľl 0.2-5 Âľl No. of samples/plate 15-20 40-50 Reproducibility of results Difficult Reproducible
  • 16. High Performance Liquid Chromatography (HPLC) Principle • Highly sensitive separation technique • Sample and purified mobile phase are applied to the column under high pressure • Sample compounds are separated based on adsorption, partition, ion exchange, molecular exclusion or affinity principle
  • 17. HPLC • Relies on pumps to pass a pressurized liquid solvent containing the sample mixture through a column filled with a solid adsorbent material • Each component in the sample interacts differently with the adsorbent material
  • 18. HPLC • Different flow rates for different components lead to separation of components as they flow out of the column • Separate the complex mixture and recognize the role of individual molecules
  • 19. HPLC
  • 20. Detectors in HPLC • Choice of detectors is critical to guarantee that all the components are detected • Common types of detectors – UV detector – Photodiode array (PDA) detector – Refractive index detector – Fluorescence detector
  • 21. UV detector • Capable of monitoring several wavelengths concurrently • Can detect all the UV-absorbing components
  • 23. Photodiode array (PDA) detector • Can sense a range of wavelengths concurrently • Wavelength range can be programmed and all the compounds that absorb within this range can be identified in a single analysis
  • 25. Refractive index detector • Detector of choice to detect analytes with restricted or no UV absorption such as alcohols, sugars, carbohydrates, fatty acids, and polymers
  • 26.
  • 27. Fluorescence detector • Most sensitive detectors • 10-100 times higher than UV detector for strong UV absorbing materials
  • 29. Applications of HPLC • Manufacturing (e.g. during the production process of pharmaceutical and biological products) • Legal (e.g. detecting performance enhancement drugs in urine) • Research (e.g. separating the components of a complex biological sample) • Medical (e.g. detecting Vitamin D levels in blood serum)
  • 30. Limitations of HPLC • Price of columns and solvents • Lack of long term reproducibility due to proprietary nature of column packing
  • 31. Gas Chromatography Principle • Used in analysis of the compounds that can be vaporized without decomposition • Testing the purity of a particular substance • Separating the different components of mixture
  • 32. • Mobile phase is a carrier gas, usually an inert gas such as helium or an unreactive gas such as nitrogen • Stationary phase is a microscopic layer of liquid or polymer on an inert solid support • Gaseous compounds being analyzed interact with the walls of column Gas Chromatography
  • 34. Applications of Gas Chromatography • Assay of isotretinoin, cocaine and residual solvents in betamethasone, • Analysis of impurities of pharmaceuticals • Identification of functional group of compounds
  • 35. Spectroscopy • Analytical techniques used for quantification, characterization and structural analysis of macromolecules by measuring the absorption, transmission, emission of radiation by the molecules
  • 36. Spectroscopic techniques • UV-visible spectroscopy • Mass spectrometry • Near infrared spectroscopy • Nuclear magnetic resonance spectroscopy • Fluorimetry • Phosphorimetry
  • 38. Beer’s Law • Amount of light absorbed by a colored solution is proportional to the concentration of the solution A Îą C A = absorbance C = concentration of the color in the solution
  • 39. Lambert’s Law • Amount of light absorbed by a colored solution is proportional to the depth through which the light passes in the solution A Îą L A = absorbance L = depth through which light passes in the solution
  • 40. Colorimetry • Quantification of colored compounds in solution Irradiating with visible light (400 – 700 nm) Measuring the absorbance
  • 42. UV- Visible Spectrophotometry • Quantification and characterization of colorless compounds Irradiating with UV (185-400 nm) or visible light (400-700 nm) Measuring the absorbance
  • 45. Applications of UV-visible Spectroscopy • To quantify protein, carbohydrates, Hb, Chlorophyll • To detect impurity in biological compounds (Impurities are displayed as additional peaks in spectrum)
  • 46. Common Drugs analyzed by UV- visible spectrophotometry • Acetaminophen, Amlodipine, Ampicillin, amoxycillin, Lisinopril, Flunarizine, Carbenicillin, Diclofenac sodium, Diltiazem, Nicorandil, Pantoprazole sodium, Zidovudine, Verapamil
  • 47. Mass Spectrometry Principle • Sample is ionized by bombarding it with high energy electrons • Some of the sample’s molecules to break into charged fragments • These ions are then separated according to their mass-to-charge ratio
  • 48. Mass Spectrometry (MS) • Ions of the same mass-to-charge ratio will undergo the same amount of deflection • The ions are detected by electron multiplier which can detect charged particles • Results are displayed as spectra
  • 49. Application of MS • Elucidation of structure of organic and biological molecules • Determination of molecular mass of peptides, proteins and oligonucleotides • Identification of drugs abuse and metabolite of drugs of abuse in blood, urine and saliva
  • 50. Principle • Uses light over the infrared range (700-15000 nm) of electromagnetic radiation spectrum • The energy curve of an oscillating molecule is affected by intramolecular interactions • Vibrations around the equilibrium position are non-symmetric and the spacings between energy levels that the molecule can attain are not identical Near Infrared spectroscopy (NIRS)
  • 51. • Easy preparation without any pretreatments • Identification and qualification of raw materials and intermediates • Analysis of intact dosage forms • Process monitoring and process control Applications of (NIRS)
  • 53. Nuclear magnetic resonance spectroscopy (NMR) Principle • The important property of nucleus is spinning • Compound is subjected to external magnetic field and radio wave • Nucleus is promoted to higher magnetic energy level and resonance occurs NMR signal recorded as NMR peak gives structural information about the compound
  • 54.
  • 55. Applications of NMR • To study the structure of antibiotics, interleukin and nucleic acids • To study drug metabolism • For conformational analysis of macromolecules
  • 56. Fluorimetry Principle • Fluorescence is a phenomenon of emission of radiation when the molecules are excited by radiation at certain wavelength • Fluorimetry measures the fluorescence intensity at a particular wavelength with the help of a filter fluorimeter
  • 59. Applications of Fluorimetry • High sensitive technique to identify the presence and amount of specific molecules • Quantitative analysis of various drugs in dosage forms and biological fluids
  • 60. Phosphorimetry Principle • Phosphorescence is also a phenomenon of emission of radiation when the molecules are excited by radiation at certain wavelength • Difference from fluorimetry – emission of radiation continues after light source is cut off • Applications – Analysis of Quinolone, Riboflavin, Anticancer drugs, Naproxen
  • 61. Capillary Electrophoresis Principle • Separation of compounds that are capable of acquiring electric charge in conduction electrodes • Based on difference in migration of charged particle through a solution under the influence of an external electrical field
  • 62. Capillary Electrophoresis • Solutes are perceived as peaks as they pass through detector and the area of individual peak is proportional to concentration • Quicker time scale, requirement of only a small amount up to Nano liter injection volumes • Applications – Separation of Atropine sulphate, Codeine phosphate, Ketamine HCL, Phenylephrine HCL
  • 65. Hyphenated techniques • Provides more information than could be obtained by using the individual techniques in isolation • Time saving • Additional information
  • 66. Hyphenated techniques • Hyphenated techniques combine chromatographic and spectral methods to exploit the advantages of both • Chromatography produces pure or nearly pure fractions of chemical components in a mixture • Spectroscopy produces selective information for identification using standards or library spectra
  • 67. • GC-MS Gas chromatography–mass spectrometry • LC-MS Liquid chromatography–mass spectrometry • LC-IR Liquid chromatography–Infrared Spectroscopy • LC-NMR Liquid chromatography–Nuclear magnetic resonance spectroscopy • CE-MS Capillary electrophoresis–mass spectrometry Hyphenated techniques
  • 68. GC-MS • Compounds that are adequately volatile, small and stable in high temperature in GC conditions can be easily analyzed by GC-MS • A carrier gas propels the sample down the column • GC separates the components of a mixture in time • MS detector provides information that aids in the structural identification of each component
  • 69. LC-MS • Separated sample emerging from the column can be identified on the basis of its mass spectral data • Combines chemical separating power of LC with the ability of MS to selectively detect and confirm molecular identity
  • 70. LC-IR • Coupling of LC and detection method infrared spectrometry (IR) • IR is useful spectroscopic technique for identification of organic compounds
  • 71. LC-NMR • Analysis of complex mixtures of all types, particularly the analysis of natural products and drug-related metabolites in biofluids • Reversed-phase columns are used in LC-NMR
  • 72. CE-MS • Almost all molecules can be separated using this powerful method • Separates species by applying voltage across buffer-filled capillaries • Generally used for separating ions that move at different speeds when voltage is applied, depending on their size and charge
  • 73. References • Julia C Drees, Alan H B Wu. Analytical techniques. In: Michael L Bishop, editor. Clinical chemistry. 5th Ed, Lippincott Williams & Wilkins 2010; 130-165. • Glen L Hortin, Bruce A Goldberger. Chromatography and Extraction. In: Tietz Textbook of Clinical Chemistry and Molecular Diagnostics. 5th Ed, Elsevier 2012; 307-328.