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Electrochromatography - A Hybrid Separation Technique

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Title: Electrochromatography - A Hybrid Separation Technique

1
Electrochromatography - A Hybrid Separation
Technique

2
The Idea

Combine the attributes of size exclusion
chromatography (gel filtration chromatography)
with the benefits of gel electrophoresis.
The two separation mechanisms both operate along
the length of a gel filtration chromatography
column which has an electric field gradient
applied to the column.
Useful for the separation of large biomolecules
separated by size due to the gel filtration
mechanism
separated by electrophoretic mobility (gel
electrophoresis)
Also other chromatographic solute retention
mechanisms

3
The Basics - Gel Filtration or Permeation

Size exclusion chromatography (SEC)
particles are separated based on hydrodynamic
volume
aqueous mobile phase gel filtration
chromatography
organic mobile phase gel permeation
chromatography
widely applied for purification and analysis of
synthetic or bio-polymers (proteins,
polysaccharides, nucleic acids)
biopolymers - use a gel stationary phase (usually
polyacrylamide, dextran, or agarose) at low
pressures
synthetic polymers - use either a silica or
crosslinked polystyrene stationary phase at
higher pressures
Various mobile phases can be used

4
The Basics Hydrodynamic Volume

Related to the radius of gyration - measure of
the size of an object
calculated as the r.m.s. distance of the parts
(or surface) of an object from either its center
of gravity or an axis
the radius of gyration is used to describe the
dimensions of polymer chains
chain conformations of polymer samples are quasi
infinite, change over time
the "radius of gyration" discussed in polymer
physics must usually be
understood as a mean over
all polymer molecules of the
sample and over time
Rg determined experimentally with static light
scattering as well as with small angle neutron-
and x-ray scattering.
The hydrodynamic radius is numerically similar,
and can be measured with size exclusion
chromatography.

5
SEC Illustrated
6
Gel Filtration or Permeation Inst.

7
Standard Gel Electrophoresis

Separation uses a gel" as the stationary phase
it is often a crosslinked polymer
For proteins or small nucleic acids (DNA, RNA, or
oligonucleotides) the gel is usually composed of
acrylamide and a cross-linker (in various ratios)
producing mesh networks of polyacrylamide with
different sized pores.
For larger nucleic acids (greater than a few
hundred bases), agarose is the preferred matrix.
"Electrophoresis" refers to the electromotive
force (EMF) that is used to move the molecules
through the gel matrix.
the molecules move through the matrix at
different rates,
usually determined by mass,
Motion is toward the positive anode if negatively
charged or toward the negative cathode if
positively charged

8
The Basics Cap. Electrophoresis

Capillary electrophoresis (CE), also known as
capillary zone electrophoresis (CZE)
used to separate ionic species by their charge
and frictional forces.
traditional electrophoresis, electrically charged
analytes move in a conductive liquid medium under
the influence of an electric field
Introduced in the 1960s, the technique of
capillary electrophoresis (CE) was designed to
separate species based on their size to charge
ratio in the interior of a small capillary filled
with an electrolyte

9
The Basics Electrophoretic Mobility

analyte electrophoretic migration velocity (up)
toward the electrode of opposite charge is
up µpE
µp electrophoretic mobility
E is the electric field strength
electrophoretic mobility at a given pH
z is the net charge of the analyte
the viscosity (?) of the medium
r is the Stokes radius of the analyte
D is the diffusion coefficient.

10
The Basics electroosmotic flow

EOF does not significantly contribute to band
broadening as in pressure-driven chromatography.
Capillary electrophoresis separations can have
several hundred thousand theoretical plates

11
The Basics electroosmotic flow

electroosmotic flow (EOF) of buffer is directed
toward the cathode (-)
the electroosmotic flow of buffer gt
electrophoretic flow of the analytes
all analytes are carried along with the buffer
toward the cathode
analytes do migrate toward the electrode of
opposite charge
negatively charged analytes attracted to anode
(), counter to the EOF
positively charged analytes attracted to cathode
(-) with the EOF
anionic analytes retained longer due to
conflicting electrophoretic mobilities
small multiply charged cations migrate quickly
and small multiply charged anions are retained
strongly

12
The Instrumental Requirements

13
Electrochromatography

high efficiency of CE is combined with the high
selectivity of micro-HPLC
hybrid technique known as capillary
electrochromatography (CEC).
utilizes columns similar to those used in
micro-HPLC
the mobile phase is driven by an electric
potential as in CE
separation mechanism is the result of the
combination of chromatographic partitioning and
electrophoretic migration.
CEC can be done in a CE instrument with a
micro-HPLC column

14
Electrochromatography
15
Electrochromatography

16
Gradient Electrochromatography
17
Gradient Electrochromatography

Separation of 16 PAHs
Column EP-75-26-3-C18. Voltage 20kV for the
isocratic separations. Injection 5kV/5s.
Detection LIF, ex 257nm, em 400nm.
Sample
1. naphthalene, 2. acenaphthylene,
3. acenaphthene, 4. fluorene,
5. phenanthrene, 6. anthracene,
7. benzobfluoranthene,
8. pyrene,
9. benzaanthracene,
10. chrysene,
11. benzobfluoranthene,
12. benzokfluoranthene,
13. benzoapyrene,
14. dibenza,hanthracene,
15. benzoghiperylene, and
16. indeno1,2,3-cdpyrene.