ABOUT HPLC

1. INSTRUMENTATION OF HPLC
Presented by:
SK.SAMIYA,
Dept. of Pharmacology.

2. CONTENTS
 Introduction
 Types
 Instrumentation
 Advantages
 Disadvantages
 Applications

3. INTRODUCTION
 HPLC- High Performance Liquid Chromatography
Or
High pressure liquid chromatography
Definition:
 It is a chromatographic technique used to separate components of
mixture for the purpose to identify, quantify or purify the individual
components of the mixture.
 This is widely used in field of biochemistry and analytical chemistry.

4. Types of HPLC techniques
 Based on mode of chromatography
 Based on principle of separation
 Based on elution technique
 Based on scale of operation
 Based on type of analysis

5. Based on modes of chromatography
Normal phase mode:
 The stationary phase is polar in nature & the mobile phase is non-
polar.
 This is not advantageous in pharmaceutical application since most of
the drug molecules are polar in nature and takes longer time to be
eluted and detected.
Reverse phase:
 The stationary phase is non-polar & the mobile phase is polar in
nature.
 Since most of the drugs and pharmaceuticals are polar in nature, they
are not retained for a longer time and eluted faster.

6. Based on principle of separation
 Adsorption chromatography: Separation of components takes place
because of the difference in affinity of compounds towards stationary
phase.
 Ion exchange chromatography: An ion is used to separate a mixture
of similar charged ions.
 Size exclusion or gel permeation chromatography: A mixture of
components with different molecular sizes are separated by using gels
which acts as sieve.

7. Based on elution technique
 Isocratic separation: In this technique, the same mobile phase
combination is used throughout the process of separation. The same
polarity or elution strength is maintained throughout the process.
 Gradient separation: In this technique, a mobile phase combination
of lower polarity or elution strength is used followed by gradually
increasing the polarity or elution strength.

8. Based on the scale of operation
 Analytical HPLC: Where only analysis of the samples are done.
Recovery of the samples is not done
 Preparative HPLC: Where the individual fractions of pure
compound can be collected using fraction collector. The collector
samples are reused.

9. Based on the type of analysis
 Qualitative analysis: Which is used to identify the compound, detect
the impurities, to find the number of components, etc
 Quantitative analysis: Which is done to determine the quantity of
the individual or several components in a mixture. This can be done
by comparing peak area of the standard and sample

10. INSTRUMENTATION
HPLC instrument consists of following components:
 Pump
 Mixing unit
 Solvent degassing
 Injector
 Column
 Detectors
 Application

13. PUMP
 The role of the pump is to force a liquid ( called the mobile phase)
through the liquid chromatography at a specific flow rate, expressed
in milliliters per min (mL/min)
 Normal flow rates in HPLC are in the 1-2mL/min range.
 During the chromatographic experiment, a pump can deliver a
constant mobile phase composition (isocratic) or an increasing mobile
phase composition (gradient).
 Best for the analysis of complex samples.

14. Types of pumps:
Mainly three types:
• Constant flow reciprocating pump
• Syringe type pump
• Pneumatic pump

15. Constant flow reciprocating pump
 The term reciprocating describes
any continuously repeated
backwards and forwards motion.
 Widely used type of pump.
 Solvent is sucked during back
stroke and gets deliver to the
column in forward stroke.

16. Syringe or displacement type pump
 Consists of large syringe like chamber.
 Suitable for small bore column.

17. Pneumatic pump
 Gas is used to pressurize the mobile phase present in a collapsible
solvent container.

18. MIXING UNIT
 Mixing unit is used to mix solvents in different proportions and pass
through the column.
 There are two types of mixing units.
- they are low pressure mixing chamber which uses helium for
degassing solvents.
- high pressure mixing chamber does not require helium for degassing
solvents
 Mixing of solvent is done either with a static mixer which is packed
with beads or a dynamic mixer which uses magnetic stirrer and
operates under high pressure.

19. SOLVENT DEGASSING
 Several gases are soluble in organic solvents.
 When solvents are pumped under high pressure, gas bubbles are
formed which will interfere with the separation process, steady
baseline and the shape of the peak.
 Hence degassing is necessary.

20. This can be done by using following techniques:
 Vacuum filtration:- which can remove air bubbles, but it is not always
reliable and complete.
 Helium purging:- By passing helium through the solvent. This is very
effective but expensive.
 Ultrasonification:- By using Ultrasonicator, which converts ultra high
frequency to mechanical vibrations. This causes the removal of air
bubbles.

21. INJECTOR
 The injector serves to introduce the liquid sample into the flow stear
the mobile phase.
 Typical sample volumes are 5-20microliters
 The injector must also be able to withstand the high pressure of the
liquid system.
 An auto sampler is the automatic version for when the user has many
samples to analyze or when manual injection is not practical.

22. Types of injectors:
1) Septum injectors: For injecting the sample through a rubber septum.
This is not common, since the septum has to withstand high pressure.
2) Stop flow: In which the flow of mobile phase is stopped for a while and
the sample is injected through a valve device.

23. 3) Rheodyne injector: It is the most popular injector. This has a fixed
volume loop like 20µL or 50µL or more. Injector has 2 modes, i.e., load
position when the sample is loaded in the loop and inject mode when
the sample is injected.

24. COLUMN
 It is the heart of the chromatograph
Column length: varies from 5cm to 30cm
Column diameter: ranges from 2mm to 50mm
Particle size: from 1µ to 20µ
Particle nature: spherical, uniform sized, porous materials are used.

26. Materials of construction for the tubing:
 Stainless steel ( the most popular, gives high pressure
capabilities)
 Glass (mostly for biomolecules)
 PEEK (poly ether ether ketone) polymer (biocompatibility and
chemically inert to most solvents).
Packing material:
 The packing material is prepared from SILICA particle,
ALUMINA particle and ion exchange RESIN.
 Porous plug of stainless steel or Teflon are used in the end of the
columns to retain the packing material.

27. DETECTORS
 UV detectors
 Refractive index detector
 Flourimetric detector
 Conductivity detector
 Amperometric detector

28. ADVANTAGES
 Separation of volatile and non-volatile components
 Quick analysis
 High resolution
 More reproducibility
DISADVANTAGES
 High cost
 Complex to operate

29. APPLICATIONS OF HPLC
 Qualitative analysis
 Checking the impurity of a compound
 Presence of impurities
 Quantitative analysis
 Isolation and identification of drugs
 Isolation and identification of mixture of components
 Biopharmaceutical and pharmacokinetic studies
 Stability studies
 purification.