2-Step Immunoperoxidase Procedure: Epitope Retrieval Method for Formalin-fixed, Paraffin-embedded tissues and cell blocks

See the protocol steps detailing the 2-step immunoperoxidase procedure: epitope retrieval method for formalin-fixed, paraffin-embedded tissues and cell blocks method, with the reagents and procedure to successfully complete this experiment.

Materials:

Xylene
Reagent alcohol histology grade
Methanol
30% Hydrogen Peroxide
Hydrophobic barrier pen
Retrieval Buffer-Citrate Buffer pH 6.0
Retrieval Buffer-Tris-EDTA Buffer pH 9.0
Wash Solution
Normal Goat Serum Blocking Solution
IHC Antibody Diluent
Goat anti-Rabbit IgG Antibody (Bethyl cat# A120-201P, A120-401P, A120-501P)
DAB Substrate (KPL DAB Reagent Set #54-10-00)
IHC Hematoxylin
IHC Bluing Solution
Mounting media
Coverglass

Preparation of Materials:

10mM Citrate Buffer pH 6.0

2.94 g Tri-sodium Citrate (dihydrate)
Volume to 1 Liter with distilled water
Check pH (pH is usually at 6.0).
Store at room temperature for 3 months or at 4° C for 6 months.

Tris-EDTA Buffer pH9.0 (10mM Tris Base, 1mM EDTA)

1.21 g Tris Base
0.37 g EDTA
Volume to 1 Liter with distilled water
Check pH (pH is usually at 6.0).
Store at room temperature for 3 months or at 4° C for 6 months.

Methanol/H2O2 Peroxidase quench solution

6ml 30% Hydrogen peroxide
194ml Methanol. Use caution when handling and disposing methanol.
Prepare just prior to use.

Normal Goat Serum Blocking Solution

20 ml normal goat serum (Filter sterilize with 0.2 µM filter)
Volume to 100 ml with PBS or TBS.
Store 2-8 C, discard after 3 months.

IHC Antibody Diluent (50mM TBS, 1% BSA)

190 ml 1X TBS
2 g BSA (Sigma A9647)
Volume to 200 ml with TBS.
Store 2-8 C, discard after 1 year.

*May want to use a perservative.

Wash solution

Can be any of the following: PBS, TBS or 0.01% Tween 20 in dH20. TBS wash solution is recommended for phospho antibodies.

Secondary Antibody

Goat anti-Rabbit IgG Antibody-horseradish peroxidase conjugated. (Bethyl cat# A120-201P, A120-401P, A120-501P) Dilute 1:100 with IHC antibody diluent. Prepare just prior to use. Optimal working dilutions should be determined experimentally by the investigator.

DAB Solution

DAB Reagent set (KPL Cat #54-10-00)

IHC Hematoxylin

10 ml Gill 1-regular strength (StatLab #SL97-16)
90 ml distilled water

IHC Bluing Solution

50ml 10X Tris pH 7-8
450 ml distilled water

Procedure:

Xylene - 3 changes for 5 minutes each
100% Reagent alcohol - 3 changes for 5 minutes each
Methanol/H2O2 - 5-15 minutes
dH20 rinse
Place prepared Epitope Retrieval Buffer (refer to Bethyl antibody datasheet for appropriate epitope retrieval buffer) into steamer or water bath and heat to 96-100%deg; C
Add rack of slides to hot Epitope Retrieval Buffer - 20 minutes
Remove container and slides from steamer or water bath and cool on bench - 20 minutes
Slowly add dH20 for 5 minutes
dH20 rinse - 1 minute
Circle section with a hydrophobic barrier pen. Do not allow sections to dry for the remaining procedure.
Wash Solution - 3 changes for 5 minutes each
Normal Goat Serum Blocking Solution - 15 minutes
Primary Antibody Incubation: 1 hour - room temperature
- Prepare primary antibody with IHC Antibody Diluent
- Optimal working dilutions should be determined experimentally by the investigator.
- Refer to Bethyl antibody datasheet for suggested dilution range.
Wash Solution - 3 changes for 5 minutes each
Secondary Antibody Incubation: 1 hour - room temperature
Wash Solution - 3 changes for 5 minutes each
DAB development - 5-10 minutes. Monitor development with microscope. Do not develop longer than 10 minutes.
Wash Solution - 3 changes for 5 minutes each
IHC Hematoxylin - 1-3 minutes
Wash Solution - 3 changes for 5 minutes each
IHC Bluing Solution - 1-2 minutes
dH20 rinse
70% reagent alcohol - 3 minutes
95% reagent alcohol - 2 changes for 3 minutes each
100% reagent alcohol - 3 changes for 3 minutes each
Xylene - 3 changes for 3 minutes each
Mount and coverslip.
Place slides flat to dry.