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ELECTROPHORESIS
 Multiple myeloma
*a sharp distinct M band appears in -globulin fraction*
 Acute infections
*α1 and α2 globulins are increased*
 Nephrotic syndrome
*decreased albumin with sharp and prominent α2
globulin*
 primary immune deficiency
*Diminished -globulin band*
 α1-Anti trypsin deficiency
*diminished α1-globulin band*
 Waldenstrom’s macroglobulinemia
 Primary amyloidosis
 Unexplained peripheral neuropathy
 New onset anemia with renal failure
 Hypercalcemia related to malignancy
 Rouleaux formation on peripheral smear
 renal insufficiency with associated serum
protein elevation.
 Unexplained pathologic fracture or lytic lesion
on radiograph...
 CNS infections and inflammations
 Dyslipidemias
 Epidemics (micro organism causing epidemic
can be detected using PFGE)
 Drug monitoring using capillary electrophoresis
Other indications in clinical chemistry
Electrophoresis is a physical method analysis
which involves separation of the compounds
that are capable of acquiring electric charge in
conducting electrodes.
Electrophoresis may be defined as the
migration of the charged particle through a
solution under the influence of an external
electric field.
ELECTROPHORESIS
ZONE
ELECTROPHORESIS
MOVING
BOUNDARY
ELECTROPHORESIS
ZONE
ELECTROPHORESIS
PAPER
ELECTROPHORESIS
WHATMANN FILTER
PAPER
ELECTROPHORESIS
GEL
ELECTROPHORESIS
CAPILLARY
ELECTROPHORESIS
GEL ELECTROPHORESIS
AGAROSE GEL ELECTROPHORESIS
POLYACRYLAMIDE GEL ELECTROPHORESIS
SDS-PAGE
DISC ELECTROPHORESIS
ISOELECTRIC FOCUSSING
IMMUNOELECTROPHORESIS
TWO DIMENSIONAL ELECTROPHORESIS
NO SUPPORTING MEDIUM USED FOR MOVING
BOUNDARY ELECTROPHORESIS
Arne Tiselius
(10 August 1902 – 29 October1971)
Swedish biochemist
 Basic components of zone
electrophoresis…..
 supporting medium.
 Buffer chamber.
 Power pack and electrode.
 Sample dissolved in buffer tracking dye.
 Perspex cover to encase the entire chamber.
Most commonly used buffers in zone electrophoresis.
*ACETATE
*PYRIDINE
*BARBITONE
*TRIS(2-Amino,2-hydroxy methyl,1-3diol)
most commonly used
*CITRATE
Barbitone
buffer(pH-8)
• s.Protein
separation
• Poor resolution
• Week buffer
Phosphate
buffer(pH7)
• Enzymes separation
• Low buffering
capacity
• High conductivity
TRIS- BORATE –
EDTA(TBE)
(pH-8)
• Nucleic acid separation
• Good resolution &high
buffering capacity
• Low conductivity
TRIS-acetate-
EDTA(pH-8) (TAE)
• Nucleic acid
separation
• High resolution & high
buffering capacity
• Low conductivity
TRIS- glycine
buffer(pH >8)
• Protein separation
• High buffering capacity
• Low conductivity
TRIS- GLYCINE buffer
In 600 ml
distilled
water
3.6grams
TRIS
4.6
grams
GLYCINE
1
• Sample is spotted on supporting medium
2
• Medium is placed between electrodes
3
• Power pack is switched on
4
• Voltage applied till dye has travelled approx 2cm from other end
5
• Medium removed and dried
• stained with coomassie brilliant blue
6
• Destained with 5% acetic acid
7
• Bands are visualized and analyzed using densitometer
Supporting
medium
Buffer
Electric
current
Size,shape &net
charge of molecule
Heat and
electroendosmosis
 Paper electrophoresis is mainly used for separation of
protein(at low voltage), amino acids and nucleotides(at
high voltage).
 Greatest disadvantage of paper electrophoresis is
diffusion, adsorption and electroendosmosis.
 To over come these issues high voltage is applied 10,000
volts that results in good resolution and rapid separation.
 Small molecules like amino acids and nucleotides are
separated by high voltage electrophoresis
Paper electrophoresis
 General procedure is similar to that of paper electrophoresis
 Cellulose acetate electrophoresis has replaced paper
electrophoresis
 Better resolution in short time.
 Negligible adsorption and EEO
 Suitable for fractionation of polysaccharides and lipoproteins
 Bands are easily detected due to transparency of medium.
Cellulose acetate Electrophoresis
 Separation of DNA using constant electric field is called
constant field gel electrophoresis(CFGE).
 Separation of DNA altering the strength and direction of
electric field between the electrodes is called as pulse
field gel electrophoresis(PGFE)
 PGFE used to separate high molecular weight DNA.
 CFGE is normal agarose gel electrophoresis for
molecular weight up to 500kb.
 PGFE used to separate human chromosome and yeast
chromosome with sharper bands and high resolution.
 Polyacrylamide gels are used for protein fractionation in the presence of
SDS(sodium dodecyl sulphate)
 Polyacrylamide could be used in the form of tube gel(for small volume of
samples)
 Vertical slab gel (for large volume of samples)
 Denaturing of protein sample is needed because protein structure is stable with
hydrophobic interaction, hydrogen bond, and disulphide bond.
 Stable structure does not favour electrophoresis and need to disturb its
structure
 Denaturing agents SDS, urea, and beta mercaptoethanol
Denatured
sample
loaded
Running
buffer
(TRIS-
GLYCINE)
ph8.8
80volts
current
applied&
allow it till it
reach 5cm
above lower
end
Staining by
coomassie or
silver staining
Destaining
using
methanol,
acetic acid,
water
mixture
Determine molecular weight of proteins
To fractionate protein subunits
To assess the purity of proteins samples
Native PAGE with out SDS
 To separate enzymes and isoenzymes
Disc electrophoresis(tube electrophoresis)
 Tank of 100 ml buffer forms anode above and another tank of
100 ml forms cathode below.
 Six holes of 2mm diameter are drilled1.5 cm apart and 1mm
above the buffer.
 Any protein specimen can be fractioned using this apparatus.
 The order of resolution is prealbumin, albumin , postalbumins
, ceruloplasmin ,transferrin, post transferrin fractions and
gamma- globulins.
 Lipoproteins separation and studies on Isoenzymes were also
carried out using this apparatus.

Disc electrophoresis
(tube electrophoresis)
 IEF is a type of gel electrophoresis in which
compounds are separated in a gel with ph gradient ,
based on differences in iso electric point.
 IEF gel has pre selected pH range.
 Compounds with pH less than iso electric pH acquire
negative charge and move towards anode and vice
versa move towards cathode.
 Migration continues till the molecules reach a pH
region in the gel, which is equal to their iso electric
point.
 At that point molecules become stationary and exist
as zwitter ions.
Isoelectric focusing
 To determine iso electric point of protein.
 To separate iso enzymes.
 To fractionate proteins with higher resolution.
 To separate all amphoteric substances.
 To study mono,di,tri substituted derivatives of
proteins.
In 2D PAGE, the molecules are first separated by IEF
in a gradient gel, and then by SDS PAGE in a second
gel.
2D PAGE IS USED:
*To resolve proteins and enzymes with high resolution
*To assess purity of proteins.
Molecules separated
by…
• pH gradient gel
cast on narrow
cylindrical tube
Gel extruded from
tube…
• Incubated in SDS for
30 min to denature
the protein
Placed on second gel
and stacking gel,
voltage applied and
protein sub units are
separated
 IEF combines sensitivity of gel electrophoresis
and specificity of immune reaction.
 This technique is used to quantify antigen.
 In capillary electrophoresis, separation is done
with in capillary tube under high pressure and
high voltage to give better resolution in short
time
 To separate amino acids.
 To separate oligonucleotides and nucleic acids.
 To separate drugs.
 To separate metal ions.
 To separate enantiomers.
 Is used for fractionation of both DNA and
protein
 But with different buffers and at different
current and voltages.
 Agarose gel is used as supporting medium
which is a polysaccharide derivative of agar.
 The pores of agarose gel act as molecular
sieve.
 Pore size of gel is inversely proportional to the
initial concentration of agarose
 0.8% of agarose used for DNA of 0.5-10kb.
1% AGAROSE
100MG
WEIGHED AND
TAKEN IN TO
TEST TUBE
Place the test tube in boiling water bath for
about 10minutes
After taking out from water
bath evenly mixed agarose
gel taken in to pipette…….
POUR THE BUFFER IN TO THE
TANK and connect wicks
Run power pack for 1.30 hours at 150volts for
better results
For a period of 30 minutes
leave the slide in the fixative
Can use drier or hot air oven
Dry the slide till the agarose
fixes to slide
Made to 100ml (CBB dye)
Glacial
acetic
acid 7ml
Dye
300mg
Ethanol
50ml
Leave the slide in the
CBB stain for 30
minutes
Normal serum pattern
Nephrotic syndrome
Increased albumin Decreased albumin
• dehydration • Chronic cachectic or wasting
diseases
• Chronic infections
• hemorrhage
• burns
• Protein loosing enteropathies
• Impaired liver function
• malnutrition
• Nephrotic syndrome
Increased α1 globulins Decreased α1 globulins
pregnancy α 1 antitrypsin deficiency
Increased α2 globulins Decreased α2 globulins
Adrenal insufficiency malnutrition
Adrenocorticosteroid therapy Megaloblastic anaemia
Diabetes mellitus Protein losing enteropathy
Nephrotic syndrome Severe liver disease
Wilson’s disease
increasedβ1 or β2
globulins
decreasedβ1 or β2
globulins
Biliary cirrhosis Protein malnutrition
carcinomas
Cushings disease
Diabetes mellitus
hypothyroidism
Iron deficiency anemia
Malignant hypertension
nephrosis
Poly arteritis
Obstructive jaundice
Increased -globulins Decreased -globulins
 amloidosis  Agamma globulinemia
 Chronic infections  hypogammaglobulinemia
 Chronic lymphocytic luekemia
 cirrhosis
 Hodgkin’s diseases
 Malignant lymphoma
 Multiple myeloma
 Connective tissue disorders
 Waldenstrom’s
macroglobulinemia
Electrophoresis for pgs by Dr siva kumar reddy

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Electrophoresis for pgs by Dr siva kumar reddy

  • 2.  Multiple myeloma *a sharp distinct M band appears in -globulin fraction*  Acute infections *α1 and α2 globulins are increased*  Nephrotic syndrome *decreased albumin with sharp and prominent α2 globulin*  primary immune deficiency *Diminished -globulin band*  α1-Anti trypsin deficiency *diminished α1-globulin band*
  • 3.  Waldenstrom’s macroglobulinemia  Primary amyloidosis  Unexplained peripheral neuropathy  New onset anemia with renal failure  Hypercalcemia related to malignancy  Rouleaux formation on peripheral smear  renal insufficiency with associated serum protein elevation.
  • 4.  Unexplained pathologic fracture or lytic lesion on radiograph...  CNS infections and inflammations  Dyslipidemias  Epidemics (micro organism causing epidemic can be detected using PFGE)  Drug monitoring using capillary electrophoresis Other indications in clinical chemistry
  • 5. Electrophoresis is a physical method analysis which involves separation of the compounds that are capable of acquiring electric charge in conducting electrodes.
  • 6. Electrophoresis may be defined as the migration of the charged particle through a solution under the influence of an external electric field.
  • 9. GEL ELECTROPHORESIS AGAROSE GEL ELECTROPHORESIS POLYACRYLAMIDE GEL ELECTROPHORESIS SDS-PAGE DISC ELECTROPHORESIS ISOELECTRIC FOCUSSING IMMUNOELECTROPHORESIS TWO DIMENSIONAL ELECTROPHORESIS
  • 10. NO SUPPORTING MEDIUM USED FOR MOVING BOUNDARY ELECTROPHORESIS Arne Tiselius (10 August 1902 – 29 October1971) Swedish biochemist
  • 11.  Basic components of zone electrophoresis…..  supporting medium.  Buffer chamber.  Power pack and electrode.  Sample dissolved in buffer tracking dye.  Perspex cover to encase the entire chamber.
  • 12. Most commonly used buffers in zone electrophoresis. *ACETATE *PYRIDINE *BARBITONE *TRIS(2-Amino,2-hydroxy methyl,1-3diol) most commonly used *CITRATE
  • 13. Barbitone buffer(pH-8) • s.Protein separation • Poor resolution • Week buffer Phosphate buffer(pH7) • Enzymes separation • Low buffering capacity • High conductivity TRIS- BORATE – EDTA(TBE) (pH-8) • Nucleic acid separation • Good resolution &high buffering capacity • Low conductivity
  • 14. TRIS-acetate- EDTA(pH-8) (TAE) • Nucleic acid separation • High resolution & high buffering capacity • Low conductivity TRIS- glycine buffer(pH >8) • Protein separation • High buffering capacity • Low conductivity
  • 15. TRIS- GLYCINE buffer In 600 ml distilled water 3.6grams TRIS 4.6 grams GLYCINE
  • 16. 1 • Sample is spotted on supporting medium 2 • Medium is placed between electrodes 3 • Power pack is switched on 4 • Voltage applied till dye has travelled approx 2cm from other end 5 • Medium removed and dried • stained with coomassie brilliant blue 6 • Destained with 5% acetic acid 7 • Bands are visualized and analyzed using densitometer
  • 18.
  • 19.  Paper electrophoresis is mainly used for separation of protein(at low voltage), amino acids and nucleotides(at high voltage).  Greatest disadvantage of paper electrophoresis is diffusion, adsorption and electroendosmosis.  To over come these issues high voltage is applied 10,000 volts that results in good resolution and rapid separation.  Small molecules like amino acids and nucleotides are separated by high voltage electrophoresis Paper electrophoresis
  • 20.
  • 21.  General procedure is similar to that of paper electrophoresis  Cellulose acetate electrophoresis has replaced paper electrophoresis  Better resolution in short time.  Negligible adsorption and EEO  Suitable for fractionation of polysaccharides and lipoproteins  Bands are easily detected due to transparency of medium. Cellulose acetate Electrophoresis
  • 22.  Separation of DNA using constant electric field is called constant field gel electrophoresis(CFGE).  Separation of DNA altering the strength and direction of electric field between the electrodes is called as pulse field gel electrophoresis(PGFE)  PGFE used to separate high molecular weight DNA.  CFGE is normal agarose gel electrophoresis for molecular weight up to 500kb.  PGFE used to separate human chromosome and yeast chromosome with sharper bands and high resolution.
  • 23.
  • 24.  Polyacrylamide gels are used for protein fractionation in the presence of SDS(sodium dodecyl sulphate)  Polyacrylamide could be used in the form of tube gel(for small volume of samples)  Vertical slab gel (for large volume of samples)  Denaturing of protein sample is needed because protein structure is stable with hydrophobic interaction, hydrogen bond, and disulphide bond.  Stable structure does not favour electrophoresis and need to disturb its structure  Denaturing agents SDS, urea, and beta mercaptoethanol
  • 25.
  • 26. Denatured sample loaded Running buffer (TRIS- GLYCINE) ph8.8 80volts current applied& allow it till it reach 5cm above lower end Staining by coomassie or silver staining Destaining using methanol, acetic acid, water mixture
  • 27. Determine molecular weight of proteins To fractionate protein subunits To assess the purity of proteins samples Native PAGE with out SDS  To separate enzymes and isoenzymes
  • 28.
  • 30.  Tank of 100 ml buffer forms anode above and another tank of 100 ml forms cathode below.  Six holes of 2mm diameter are drilled1.5 cm apart and 1mm above the buffer.  Any protein specimen can be fractioned using this apparatus.  The order of resolution is prealbumin, albumin , postalbumins , ceruloplasmin ,transferrin, post transferrin fractions and gamma- globulins.  Lipoproteins separation and studies on Isoenzymes were also carried out using this apparatus.  Disc electrophoresis (tube electrophoresis)
  • 31.
  • 32.  IEF is a type of gel electrophoresis in which compounds are separated in a gel with ph gradient , based on differences in iso electric point.  IEF gel has pre selected pH range.  Compounds with pH less than iso electric pH acquire negative charge and move towards anode and vice versa move towards cathode.  Migration continues till the molecules reach a pH region in the gel, which is equal to their iso electric point.  At that point molecules become stationary and exist as zwitter ions. Isoelectric focusing
  • 33.  To determine iso electric point of protein.  To separate iso enzymes.  To fractionate proteins with higher resolution.  To separate all amphoteric substances.  To study mono,di,tri substituted derivatives of proteins.
  • 34. In 2D PAGE, the molecules are first separated by IEF in a gradient gel, and then by SDS PAGE in a second gel. 2D PAGE IS USED: *To resolve proteins and enzymes with high resolution *To assess purity of proteins.
  • 35. Molecules separated by… • pH gradient gel cast on narrow cylindrical tube Gel extruded from tube… • Incubated in SDS for 30 min to denature the protein Placed on second gel and stacking gel, voltage applied and protein sub units are separated
  • 36.
  • 37.  IEF combines sensitivity of gel electrophoresis and specificity of immune reaction.  This technique is used to quantify antigen.
  • 38.  In capillary electrophoresis, separation is done with in capillary tube under high pressure and high voltage to give better resolution in short time
  • 39.  To separate amino acids.  To separate oligonucleotides and nucleic acids.  To separate drugs.  To separate metal ions.  To separate enantiomers.
  • 40.  Is used for fractionation of both DNA and protein  But with different buffers and at different current and voltages.  Agarose gel is used as supporting medium which is a polysaccharide derivative of agar.  The pores of agarose gel act as molecular sieve.  Pore size of gel is inversely proportional to the initial concentration of agarose  0.8% of agarose used for DNA of 0.5-10kb.
  • 42.
  • 43. Place the test tube in boiling water bath for about 10minutes
  • 44. After taking out from water bath evenly mixed agarose gel taken in to pipette…….
  • 45.
  • 46.
  • 47.
  • 48. POUR THE BUFFER IN TO THE TANK and connect wicks
  • 49. Run power pack for 1.30 hours at 150volts for better results
  • 50. For a period of 30 minutes leave the slide in the fixative
  • 51. Can use drier or hot air oven Dry the slide till the agarose fixes to slide
  • 52. Made to 100ml (CBB dye) Glacial acetic acid 7ml Dye 300mg Ethanol 50ml
  • 53. Leave the slide in the CBB stain for 30 minutes
  • 54.
  • 56.
  • 57.
  • 58.
  • 59.
  • 60.
  • 61.
  • 62.
  • 63.
  • 64. Increased albumin Decreased albumin • dehydration • Chronic cachectic or wasting diseases • Chronic infections • hemorrhage • burns • Protein loosing enteropathies • Impaired liver function • malnutrition • Nephrotic syndrome
  • 65. Increased α1 globulins Decreased α1 globulins pregnancy α 1 antitrypsin deficiency
  • 66. Increased α2 globulins Decreased α2 globulins Adrenal insufficiency malnutrition Adrenocorticosteroid therapy Megaloblastic anaemia Diabetes mellitus Protein losing enteropathy Nephrotic syndrome Severe liver disease Wilson’s disease
  • 67. increasedβ1 or β2 globulins decreasedβ1 or β2 globulins Biliary cirrhosis Protein malnutrition carcinomas Cushings disease Diabetes mellitus hypothyroidism Iron deficiency anemia Malignant hypertension nephrosis Poly arteritis Obstructive jaundice
  • 68. Increased -globulins Decreased -globulins  amloidosis  Agamma globulinemia  Chronic infections  hypogammaglobulinemia  Chronic lymphocytic luekemia  cirrhosis  Hodgkin’s diseases  Malignant lymphoma  Multiple myeloma  Connective tissue disorders  Waldenstrom’s macroglobulinemia