M.

PRASAD NAIDU
Msc Medical Biochemistry,
Ph.D Research scholar.

1. Introduction
2. Retention Mechanisms in Liquid Chromatography
3. Method Development
LIQUID
CHROMATOGRAPHY
Liquid Chromatography

Liquid Chromatography (LC) is a chromatographic technique in which the mobile
phase is a liquid.

LC is a much older technique than GC, but was overshadowed by the rapid
development of GC in the 1950s and 1960s.

LC is currently the dominate type of chromatography and is even replacing GC in
its more traditional applications.

Advantages of LC compared to GC:

LC can be applied to the separation of any compound that is soluble in a liquid phase.

LC more useful in the separation of biological compounds, synthetic or natural
polymers, and inorganic compounds

Liquid mobile phase allows LC to be used at lower temperatures than required by GC

LC better suited than GC for separating compounds that may be thermally labile
Advantages of LC compared to GC (continued):
Retention of solutes in LC depend on their interaction with both the mobile phase
and stationary phase.

GC retention based on volatility and interaction with stationary phase
LC is more flexible in optimizing separations change either stationary or mobile
phase

Most LC detectors are non-destructive

most GC detectors are destructive
LC is better suited for preparative or process-scale separations

Disadvantage of LC compared to GC:
LC is subject to greater peak or band-broadening. RESOLUTION!!!!
much larger diffusion coefficients of solutes in gases vs. liquids

Low- and High-performance Liquid Chromatography:
Many types of liquid chromatography are available, based on different stationary
phase and mobile phase combinations.
- each type may be further characterized based on its overall efficiency or
performance
Low-performance liquid chromatography
LC methods that use large, non-rigid support material
particles > 40 mm in diameter

poor system efficiencies and large plate heights

such systems have the following characteristics:
broad peaks
poor limits of detection
long separation times
columns can only tolerate low operating pressures

Solvent reservoir
Column head
Column
Column packing
Porous glass plate
Column chromatography an example of the equipment used in low-performance
liquid chromatography
Sample is usually applied directly to the top of the column.
Detection is by fraction collection with later analysis of each fraction
High-performance liquid chromatography (HPLC)

LC methods that use small, uniform, rigid support material
particles < 40 mm in diameter
usually 3-10 mm in practice

good system efficiencies and
small plate heights (H!)

such systems have the following
characteristics:

narrow peaks

shorter separation times




A typical HPLC system:
- Higher operating pressures
need for mobile phase
delivery requires special
pumps and other system
components

- Sample applied using
closed system (i.e.,
injection valve)

- detection uses a flow-
through detector
Similar to GC, solutes can be eluted from a column by using either a
constant column conditions or gradient elution

Isocratic elution: use of a constant mobile phase composition to elute
solutes
simple, inexpensive
difficult to elute all solutes with good resolution in a reasonable
amount of time general elution problem

Gradient elution: changing the composition of the mobile phase with time

solvent programming
going from a weak mobile phase to a strong one.
weak mobile phase solvent A
strong mobile phase solvent B
solvent change can be stepwise, linear or non-linear

In choosing a mobile phase for LC, several factors need to be considered
type of stationary phase used
determines what will be a strong or weak mobile phase
solubility of the solutes
viscosity of the mobile phase
type of detector used and solvent's background signal
purity of the solvents
miscibility of the solvents (for gradient elution)
Gradient elution of
mixture of 30 amino-
acids
1. Introduction
2. Retention Mechanisms in Liquid Chromatography
3. Method Development
LIQUID
CHROMATOGRAPHY
Types of Liquid Chromatography (Retention Mechanisms ):

Techniques in LC are classified according to the method of solute separation
Adsorption chromatography Affinity chromatography
Partition chromatography Size-exclusion chromatography
Ion-exchange chromatography
1. Adsorption chromatography (Liquid-solid Chromatography)
a. A LC technique which separates
solutes based on their adsorption to
an underivatized solid particles is
known as adsorption
chromatography, or liquid-solid
chromatography.
This technique is suited for non-
polar small compounds (MW<5000).
b. One advantages of adsorption chromatography, as is also true for
GSC, is that it is able to retain and separate some compounds that can
not be separated by other methods. One such application is in the
separation of geometrical isomers.
c. Mechanism
(a) Retention of solute in adsorption chromatography can be viewed
as solute A displacing n moles of solvent M from a surface.
A
mp
+ nM
sp
A
sp
+ nM
mp
2. Partition chromatography (Liquid-liquid Chromatography)
a. Partition chromatography, or liquid-liquid
chromatography is a Chromatographic
technique in which solute are separated
based on their partition between a liquid
mobile phase and a liquid stationary
phase coated on a solid support.
Phase 2
Phase 1
Phase 2
Phase 1
b. The support material used in partition chromatography is usually
silica. Un-bonded and banded stationary phase.
c. Mechanism:
The retention of solute in partition chromatography is given by:
k = K
D
(V
s
/V
m
)
d. Applications of partition Chromatography
How can ions be separated by using partition Chromatography?
Normal Phase LC and Reversed-phase LC
Stationary phase: polar non-polar
e. Ion-pair Chromatography
(b) In this method, counterions (species of opposite charge to the
solutes) thereby regulate the retention. Typically alkyl amines or
tetra alkyl amines are added to ion pair with acids whereas alkyl
sulfates, sulfonates, or phosphates are used to ion pair with bases
(a) Ion-pair chromatography is used for the separation of ionic and
ionizable compounds and mixtures of neutral and ionic
compounds.
A
-
+ B
+
A
-
B
+
3. Ion-Exchange Chromatography
a. Ion-exchange chromatography is a liquid chromatography technique in
which solutes are separated by their adsorption onto a support containing
fixed charge onto a support containing fixed charges on its surface.
b. Ion-exchange is a fairly common technique used in water softeners and in
the industrial removal or replacement of ionic compounds for products. Ion-
exchange is used in chromatography for separation of a wide variety of
charged compounds, including inorganic ions, organic ions, and biological
compounds (such as amino acids, proteins and nucleic acids)
c. Mechanism
n(supportA
-
B
+
) + C
n+
(supportA
-
)
n
C
n+
+ nB
+
K = ([B
+
]
n
[C
n+
]/[B
+
]
n
[C
n+
])
4. Affinity chromatography
Insert matrix
Antibody
Enantiomer with
Low affinity to the
antibody
Enantiomer with
high affinity to the
antibody
Antibody-antigen
For biomolecule
separation
5. Size-exclusion Chromatography for polymer and bio-
polymer
Retention of a solute is dependent on Standard entropy effect.

Diameter of the pore is very important for solute selectivity.

Multiple pore sizes should be used for separate solutes with different
sizes.
GPC: Gel permeation Chromatography (polymer scientists)
GFC: Gel filtration Chromatography (biochemists)
Standard entropy effect
K =
1-
2a
d
c
2
1. Introduction
2. Retention Mechanisms in Liquid Chromatography
3. Method Development
LIQUID
CHROMATOGRAPHY
LC Method Development
Problem Definition
Mode selection
Selectivity Optimization
System optimization
Method Validation
What type of LC should be used?
Stationary phase and mobile phase,
Temperature
Column length, particle size, flow rate,
instrument configuration, sample
injection
Accuracy, sensitivity, specificity, detection
Limit, quantification limit, linearity
Solvent
Refractiv
e Index
Viscosity
(cP)
Boiling
Point (
o
C)
Polarity
Index (P)
Eluent
Strength (e
o
)
Fluoroalkanes 1.27-1.29 0.4-2.6 50-174 <-2 -0.25
cyclohexane 1.423 0.90 81 0.04 -0.2
N-hexane 1.327 0.30 69 0.1 0.01
1-chlorobutane 1.400 0.42 78 1.0 0.26
Carbon tetrachloride 1.457 0.90 77 1.6 0.18
i-propyl ether 1.365 0.38 68 2.4 0.28
toluene 1.494 0.55 110 2.4 0.29
Diethyl ether 1.350 0.24 35 2.8 0.38
tetrahydrofuran 1.405 0.46 66 4.0 0.57
chloroform 1.443 0.53 61 4.1 0.40
ethanol 1.359 1.08 78 4.3 0.88
Ethyl acetate 1.370 0.43 77 4.4 0.58
dioxane 1.420 1.2 101 4.8 0.56
methanol 1.326 0.54 65 5.1 0.95
acetonitrile 1.341 0.34 82 5.8 0.65
nitromethane 1.380 0.61 101 6.0 0.64
Ethylene glycol 1.431 16.5 182 6.9 1.11
water 1.333 0.89 100 10.2 large
Selection of a mobile phase for a particular LC application can be done by using
various tables that summarize properties for common LC solvents:

LIKE DISSOLVES LIKE!
k
2
/k
1
= 10
(P
1
P
2
)/2
For NPLC (capacity factors):
k
2
/k
1
= 10 For RPLC (capacity factors):
(P
2
P
1
)/2



Mobile-phase selection in partition Chromatography
Example 28-1: In a reversed-phase column, a solution was found to have
A retention time of 31.3 min, while an un-retained species required 0.48 min
For elution when the mobile phase was 30% (by volume) methanol and 70% water.
Calculate (a) k , (b) a water/methanol composition that should bring k to a
value of about 5, and (c) the retention time of this solution under this new
mobile phase (assuming that the retention time of the un-retained species is
not changed).
THANK YOU