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General IHC Protocol*
Frozen Sections:| 1. | Snap frozen fresh tissues in liquid nitrogen or isopentane pre-cooled in liquid nitrogen, embedded in OCT compound in cryomolds. Store frozen blocks at -80 ºC. |
| 2. | Cut 4-8 um thick cryostat sections and mount on superfrost plus slides or gelatin coated slides. Store slides at - 80 ºC until needed. |
| 3. | Before staining, warm slides at room temperature for 30 minutes and fix in ice cold acetone for 10 minutes. Air dry for 30 minutes. |
| 4. | Wash in PBS. |
| 1. | Deparaffinize sections in xylene, 2x5min. |
| 2. | Hydrate with 100% ethanol, 2x3min. |
| 3. | Hydrate with 95% ethanol, 1min. |
| 4. | Rinse in distilled water. |
| 1. | Follow procedure for pretreatment as required. |
| 2. | Procedure for Immunoenzyme Staining. |
| 3. | Rinse Sections in Washing Buffer (PBS+0.1% Triton X-100, pH 7.4) for 2x2 min. |
| 4. | Serum Blocking: incubate sections in normal serum block – species same as secondary antibody( Wash Buffer + 5% Normal Sera). Note: since this protocol uses avidin-biotin detection system, avidin/biotin block may be needed based on tissue type. If you do, the avidin/biotin blocking should be done after normal serum block and before primary antibody incubation. |
| 5. | Primary Antibody: incubate sections in primary antibody at appropriate dilution in Wash Buffer for 1 hour at room temperature or overnight at 4C. Note:Do not rinse sections between serum block and primary antibody incubation. |
| 6. | Rinse in washing buffer for 3x2 min. |
| 7. | Peroxidase Blocking: incubate sections in peroxidase blocking solution for 10 minutes at room temperature. |
| 8. | Rinse in washing buffer for 3x2 min. |
| 9. | Secondary Antibody: incubate sections in biotinylated secondary antibody at an appropriate dilution in Wash Buffer for 30 minutes at room temperature. |
| 10. | Rinse in washing buffer for 3x2 min. |
| 11. | Detection: incubate sections in streptavidin-HRP in Wash Buffer for 30 minutes at room temperature. |
| 12. | Rinse in washing buffer for 3x2 min. |
| 13. | Chromagen/Substrate: incubate sections in peroxidase substrate solution. |
| 14. | Rinse in washing buffer for 3x2 min. |
| 15. | Rinse in running tap water for 2-5 minutes. |
| 16. | Dehydrate through 95% ethanol for 1 minute, 100% ethanol for 2x3min. |
| 17. | Clear in xylene for 2x5min. |
| 18. | Coverslip with mounting medium. |
Peroxidase Block:
0.3% H2O2 in PBS (for Paraffin Sections)
0.3% H2O2 in Methanol (for Frozen Sections)
Avidin/Biotin Block
0.001% Avidin in PBS
0.001% Biotin in PBS
Block for 10 minutes with first solution, rinse with PBS, block for 10 minutes with second solution.
*The above information is only intended as a guide. The research should determine what protocol best meets their needs. Please follow safe laboratory procedures.