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1) Eelectrophoretic separation of protein or of nucleic
acid fragments in the sample
2) Transfer to and immobilization on a matrix.
3) The probe is added to the matrix to bind to the target
molecules.
4) Any unbound probes are then removed.
5) Visualization of bound probe
Western blot
Protein Detection
• Detects proteins and estimates their molecular
weight.
• Detects changes in phosphorylation and lipid
modifications.
• Used to detect changes in protein expression.
Sample Preparation
SDS-PAGE (Protein Electrophoresis)
Electro-transferring
Immunoblotting
• Major components of the sample loading “buffer”
– SDS
– DTT
– Tracking dye
– Glycerol
– Protease inhibitor
Western Blot Visual Protocol: Phase 1: Sample Preparation
• Sodium dodecyl sulfate (SDS)
• Tris buffer (either glycine or tricine)
• Acrylamide and NN-bis-acrylamide
– Forms gel matrix
• TEMED
– Catalyst for polymerization (produces free radials from APS)
• Ammonium persulfate (APS)
– Source of free radials for polymerization
Could purchase pre-cast gels if you have the
money.
Ingredients in Gel
Stacking (concentrating) gel
4% acrylamide
0.5M Tris-H+Cl-, pH 6.8, 0.1%
SDS
Resolving (separating) gel
10% acrylamide (36.5:1,
acryl/bis)
1.5 M Tris-H+Cl-, pH 8.8, 0.1%
SDS
Running buffer
0.25 M Tris base; 1.92 M
glycine, pH 8.3; 1% SDS
Resolving gel
Stacking gel
Discontinuous system
How to Make an SDS-PAGE gel
Western Blot Visual Protocol: Phase 2: Protein Electrophoresis
• uses an electric current to pull proteins from the gel
into the PVDF or nitrocellulose membrane
• Transfer buffer contains: Tris, Glycine, and methanol
but no ions.
• Nitrocellulose membranes are cheaper than PVDF,
but are far more fragile and do not stand up well to
repeated probings
• Western blot transfer can be done in wet or semi-
dry conditions
• Equilibrate gel in transfer buffer
in separate tray.
• Equilibrate filters and sponges
in transfer buffer.
• PVDF membranes must be
soaked in methanol, before
equilibration in transfer buffer.
Nitrocellulose membranes are
soaked directly in transfer
buffer
 Mount transfer sandwich in
blotting chamber which already
contains transfer buffer
Western Blot Visual Protocol: Phase 3: Membrane Transfer
• Washing (TBS-T)
• Blocking
• Incubation with Primary antibody
• Washing (TBS-T)
• Incubation with secondary antibody
• Blocking reduces
nonspesific binding of
antibody (primary or
secondary) to protein or
membrane
• Too little => high
background
• Too much reduces the
signal
• Incubation time:
– 1-2 hrs at RT with shaking
• Blocking agents
– Fat free dry milk
– Bovin serum albumin
– Casein
– Gelatin
– Hemoglobin
– Ovalbumin
• Buffer:
– PBS, phosphate buffered saline, pH
7.5-8.0
– TBS, TRIS-buffered saline, pH 7.5
• After blocking membrane, add antibodies in to
blocking solution (ie 5% milk).
• Incubate overnight at 4oC or 2 hours at room
temperature.
• Buffer: PBS w/Tween 20 or TBS w/Tween 20
– TW20 concentration must be determined for each antibody and
antigen
– Usually 0.01-0.2%
• Time: Number of washes and duration of each wash
must be determined in each case
– Usually 3X5 min
– Use large buffer volume: 50-100 ml for 8X10 cm membrane
– Incubation with vigorous shaking
• Buffer: same as for primary antibody
• Dilution must be determined in each case
– Usually 1:1,000 - 1:100,000
• Incubation time must be determined in each case
– Varies from 5 min to 2 hrs
enzym
• Colorimetric detection
• Chemiluminescent detection
• Radioactive detection
• Fluorescent detection
Western Blot Visual Protocol: Phase 4: Immunoblotting
Protein Immunoblotting- An Introduction  to Western Blotting
Protein Immunoblotting- An Introduction  to Western Blotting

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Protein Immunoblotting- An Introduction to Western Blotting

  • 1.
  • 2.
  • 3. 1) Eelectrophoretic separation of protein or of nucleic acid fragments in the sample 2) Transfer to and immobilization on a matrix. 3) The probe is added to the matrix to bind to the target molecules. 4) Any unbound probes are then removed. 5) Visualization of bound probe
  • 5.
  • 6. • Detects proteins and estimates their molecular weight. • Detects changes in phosphorylation and lipid modifications. • Used to detect changes in protein expression.
  • 7.
  • 8. Sample Preparation SDS-PAGE (Protein Electrophoresis) Electro-transferring Immunoblotting
  • 9. • Major components of the sample loading “buffer” – SDS – DTT – Tracking dye – Glycerol – Protease inhibitor
  • 10. Western Blot Visual Protocol: Phase 1: Sample Preparation
  • 11. • Sodium dodecyl sulfate (SDS) • Tris buffer (either glycine or tricine) • Acrylamide and NN-bis-acrylamide – Forms gel matrix • TEMED – Catalyst for polymerization (produces free radials from APS) • Ammonium persulfate (APS) – Source of free radials for polymerization Could purchase pre-cast gels if you have the money. Ingredients in Gel
  • 12. Stacking (concentrating) gel 4% acrylamide 0.5M Tris-H+Cl-, pH 6.8, 0.1% SDS Resolving (separating) gel 10% acrylamide (36.5:1, acryl/bis) 1.5 M Tris-H+Cl-, pH 8.8, 0.1% SDS Running buffer 0.25 M Tris base; 1.92 M glycine, pH 8.3; 1% SDS Resolving gel Stacking gel Discontinuous system
  • 13. How to Make an SDS-PAGE gel
  • 14. Western Blot Visual Protocol: Phase 2: Protein Electrophoresis
  • 15. • uses an electric current to pull proteins from the gel into the PVDF or nitrocellulose membrane • Transfer buffer contains: Tris, Glycine, and methanol but no ions. • Nitrocellulose membranes are cheaper than PVDF, but are far more fragile and do not stand up well to repeated probings • Western blot transfer can be done in wet or semi- dry conditions
  • 16. • Equilibrate gel in transfer buffer in separate tray. • Equilibrate filters and sponges in transfer buffer. • PVDF membranes must be soaked in methanol, before equilibration in transfer buffer. Nitrocellulose membranes are soaked directly in transfer buffer  Mount transfer sandwich in blotting chamber which already contains transfer buffer
  • 17. Western Blot Visual Protocol: Phase 3: Membrane Transfer
  • 18.
  • 19.
  • 20. • Washing (TBS-T) • Blocking • Incubation with Primary antibody • Washing (TBS-T) • Incubation with secondary antibody
  • 21. • Blocking reduces nonspesific binding of antibody (primary or secondary) to protein or membrane • Too little => high background • Too much reduces the signal • Incubation time: – 1-2 hrs at RT with shaking • Blocking agents – Fat free dry milk – Bovin serum albumin – Casein – Gelatin – Hemoglobin – Ovalbumin • Buffer: – PBS, phosphate buffered saline, pH 7.5-8.0 – TBS, TRIS-buffered saline, pH 7.5
  • 22. • After blocking membrane, add antibodies in to blocking solution (ie 5% milk). • Incubate overnight at 4oC or 2 hours at room temperature.
  • 23. • Buffer: PBS w/Tween 20 or TBS w/Tween 20 – TW20 concentration must be determined for each antibody and antigen – Usually 0.01-0.2% • Time: Number of washes and duration of each wash must be determined in each case – Usually 3X5 min – Use large buffer volume: 50-100 ml for 8X10 cm membrane – Incubation with vigorous shaking
  • 24. • Buffer: same as for primary antibody • Dilution must be determined in each case – Usually 1:1,000 - 1:100,000 • Incubation time must be determined in each case – Varies from 5 min to 2 hrs enzym
  • 25. • Colorimetric detection • Chemiluminescent detection • Radioactive detection • Fluorescent detection
  • 26. Western Blot Visual Protocol: Phase 4: Immunoblotting