1. MLAB 2401: Clinical Chemistry�Keri Brophy-Martinez Electrophoresis
2. Electrophoresis Principle
the migration of charged solutes or particles in a liquid medium under the influence of an electrical field.
Distance traveled by the particle depends on its molecular weight and overall charge
Types
Iontophoresis
Migration of ions
Zone electrophoresis
Migration of macromolecules
3. Electrophoresis Clinical Application
Proteins
Immunoglobulins
Hemoglobin
Isoenzyme/enzyme
Lipoprotein
4. Components Driving force/ electrical power
Support medium
Buffer
Sample
Detecting system
5. Support Mediums Cellulose Acetate
Dry and brittle
Becomes pliable when soaked in electrolyte buffer
After electrophoresis, it can be stained and read in a densitometer
Long term storage possible
6. Support Mediums Agarose Gel
Purified agar
No electroendosmosis
After electrophoresis, it can be stained and read in a densitometer
Long term storage possible
Small sample size ~ 2-10 µL required
7. Support Mediums Polyacrylamide Gel
Gels with different pore sizes can be layered to provide good separation of molecules of different sizes
Good resolution
Detect 20 serum protein fraction rather than 5
8. Procedure Serum is applied to the support media and the protein dissolves in the buffer, giving them an electric charge
A specific amount of current is applied for a specific amount of time
As the current flows through the media, the electrically charged molecules migrate along the supporting media
9. Procedure The negatively charged protein molecules migrate towards the oppositely charged electrode
The sample is separated into bands where each band has molecules containing similar mobility
10. Staining of the Supporting Medium Staining fixes the protein to the membrane by denaturing
Makes the fractions visible
Decolorization is used to remove background color
11. Electrophoresis Bands Each peak in each column represents a different band of molecules that migrated together
Peaks with narrow bases reflect homogeneous molecules that migrate close together
Peaks with wide bases reflect heterogeneous molecules that spread out during migration
12. Densitometer A densitometer scans the stained strip and reports a graphical representation of the bands
13. Densitometer As the light beam passes through each stained band, the percent transmission is recorded and a graph representation of the concentration is recorded
A decrease in % T means the concentration of the fraction is increased and seen as a large peak on the scan
An increase in %T is graphed as a low peak or no peak
Each protein fraction can be calculated by determining the area under each peak by an intragrader
14. Factors Affecting Migration Rates Molecular weight/ size
Molecular shape
Molecular charge in the buffer
Net charge of particles
Type of supporting medium
Temperature
Electrical voltage
Migration time
15. Protein Electrophoresis
16. Relative Percent of Protein Bands
17. Common Electrophoresis Patterns
18. Hemoglobin Electrophoresis Principle and system is the same as protein electrophoresis
Solubility is an important factor in the mobility of the hemoglobin proteins
19. Hemoglobin Electrophoreis Patterns
20. References Bishop, M., Fody, E., & Schoeff, l. (2010). Clinical Chemistry: Techniques, principles, Correlations. Baltimore: Wolters Kluwer Lippincott Williams & Wilkins.
http://biotrek.rdrake.org/gallery_assorted_group_pictures.html
http://www.funsci.com/fun3_en/exper1/exper1.htm
http://themedicalbiochemistrypage.org/hemoglobin-myoglobin.html
http://science-project.com/OnlineCatalog.html
Sunheimer, R., & Graves, L. (2010). Clinical Laboratory Chemistry. Upper Saddle River: Pearson .
