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Guide IHC Staining Protocols

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Immunohistochemistry uses antibodies to detect antigens in tissue samples in order to localize proteins and study biological processes. It has various applications including cancer prognosis, tumor identification, and research. The process involves deparaffinizing tissue, antigen retrieval, blocking, primary/secondary antibody incubation, signal development using enzymes, counterstaining, and mounting slides. Different methods like direct, indirect, PAP, ABC, and LSAB are used depending on the desired sensitivity and specificity. Careful antibody selection and protocol optimization are important for obtaining high quality results.

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IMMUNOHISTOCHEMISTRY https://www.creative-bioarray.com/
CONTENTS Definition Application Method Protocol Selecting Antibody
Definition Provide quantitative, qualitative and temporal information on processes taking place in tissues. Use antibodies conjugated to enzymes that catalyze reactions to form detectable compounds to visualize and localize specific antigens in a tissue sample.The most common application of immunostaining.
Definition Antigen/Antibody based Tissue based Reaction IMMUNOHISTOCHEMISTRY
Applications of IHC οƒ˜ Prognostic markers in cancer οƒ˜ Tumors of uncertain histogenesis οƒ˜ Prediction of response to therapy οƒ˜ Infections οƒ˜ In genetics οƒ˜ Neurodegenerative disorders οƒ˜ Brain trauma οƒ˜ IHC in muscle disease οƒ˜ Research application Application
Polyclonal antibodies result in greater staining and excellent signal, but can give false positives by binding unwanted sites. Polyclonal Antibodies Monoclonal antibodies have a high specificity, reducing the number of false positive bindings, but often hive a much weaker stain. Monoclonal Antibodies Pooled monoclonal antibodies also give excellent staining and high specificity however there is limited availability for those do not bind noncompetitively. Pooled Monoclonal Antibodies Secondary antibodies, against the species of primary antibodies, will be labeled with an enzyme like HRP or biotin conjugated for staining or amplifying signal. Secondary Antibodies Selecting Antibodies
IHC Methods Direct method PAP method LSAB method Methods ABC method Indirect method
Methods β€’ One step staining method β€’ Labeled antibodies react directly with the antigen β€’ This method utilizes only one antibody and the procedure is short and quick β€’ It is insensitive due to little signal amplification and rarely used since the introduction of indirect method Direct Method Primary Antibody
Methods β€’ An unlabeled primary antibody reacts with tissue antigen β€’ A labeled secondary antibody reacts with primary antibody β€’ More sensitive due to signal amplification through several secondary antibody reactions β€’ Economy since one labeled secondary antibody can be used with many primary antibodies β€’ The secondary antibody may be labeled with enzymes or fluorescent dyes Indirect Method Primary Antibody Secondary Antibody
Methods β€’ A further development of the indirect method β€’ Involves a third layer which is a rabbit antibody to peroxidase. β€’ Bound to the unconjugated goat anti- rabbit gaba-globulin of the second layer. β€’ The sensitivity is about 100 to 1000 times higher β€’ Allows for much higher dilution of the primary antibody PAP Method Primary Antibody Secondary Antibody PAP Complex
Methods β€’ A standard IHC method β€’ The technique involves three layers. β€’ The first layer is unlabeled primary antibody. The second layer is biotinylated secondary antibody. The third layer is a complex of avidin-biotin peroxidase. β€’ The peroxidase is then developed by the DAB or other substrate to produce different colorimetric end products. ABC Method Primary Antibody Biotinylated Secondary Antibody Avidin-biotin Peroxidase Complex
Methods β€’ LSAB is similar to standard ABC method. β€’ The third layer is Enzyme-Streptavidin conjugates (HRP-Streptavidin or AP- Streptavidin) to replace the complex of avidin-biotin peroxidase. β€’ The third layer can also be Fluorescent dye-Streptavidin such as FITC- Streptavidin. β€’ Streptavidin does not contain carbohydrate groups which might bind to tissue lectins, avoiding some background staining. LSAB Method Primary Antibody Biotinylated Secondary Antibody Enzyme-Streptavidin Conjugates
Protocol οƒ˜ Dip slides in three changes of xylene for 3 minutes each. οƒ˜ Dip slides in two change of 100% alcohol for 3 minutes each. οƒ˜ Dip slides in one change of 95% alcohol for 3 minutes. οƒ˜ Dip slides in one change of 70% alcohol for 3 minutes. οƒ˜ Rinse slides twice in dH2O for 5 minutes. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Deparaffinization & Rehydration
Protocol οƒ˜ Soak slides in 3% H2O2 for 5 minutes. οƒ˜ Rinse slides twice in dH2O for 5 minutes. οƒ˜ Soak the slides in the working citrate buffer and cover with a lid. οƒ˜ Microwave until the liquid boils. οƒ˜ Remove from heat and let it stand at room temperature for 20 minutes. οƒ˜ Wash three times for 5 minutes in dH2O οƒ˜ Remove the liquid and use a PAP pen to circle around the tissue. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Antigen Retrieval
Protocol οƒ˜ Apply enough 5% BSA with a transfer pipette to cover the tissues. οƒ˜ Incubate the slides overnight at 4℃ in a humid chamber. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Bloocking
Protocol οƒ˜ Dilute the primary antibody to the recommended concentration in 1% BSA/PBS diluent. οƒ˜ Remove the BSA, and incubate with primary antibody solution for 1 hour at room temperature. οƒ˜ Wash slides three times 5 minutes each on the shaker. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Primary Antibody
Protocol οƒ˜ Dilute the biotinylated secondary antibody in 1% BSA diluent. οƒ˜ Incubate with secondary antibody solution for 30 minutes at room temperature. οƒ˜ Wash slides in PBS three times, 5 minutes each on the shaker. οƒ˜ Add enough streptavidin HRP to cover the tissues. Incubate for 30 minutes at room temperature. οƒ˜ Wash three times 5 minutes each in PBS on the shaker. οƒ˜ Add enough DAB to cover the tissues. Once the cells start turning brown, wash twice in PBS for 5 minutes each on the shaker. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Secondary Antibody
Protocol οƒ˜ Dip the slide rack with the slides into a staining dish of hematoxylin for 30 seconds. οƒ˜ Dip into an acetic bath (200mL dH2O with one to three drops of acetic acid). Rinse with dH2O. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Counterstain
Protocol οƒ˜ Dip slides in 70% and 95% alcohol for 3 minutes each. οƒ˜ Dip slides in 2 changes of 100% alcohol for 3 minutes. οƒ˜ Dip slides in 3 changes of xylene or xylene substitute for 3 minutes. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Dehydration
Protocol Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain οƒ˜ Apply coverslip to slide. οƒ˜ Let the slides dry overnight. Cover Slips Cover Slips
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Guide IHC Staining Protocols

  • 3. Definition Provide quantitative, qualitative and temporal information on processes taking place in tissues. Use antibodies conjugated to enzymes that catalyze reactions to form detectable compounds to visualize and localize specific antigens in a tissue sample.The most common application of immunostaining.
  • 5. Applications of IHC οƒ˜ Prognostic markers in cancer οƒ˜ Tumors of uncertain histogenesis οƒ˜ Prediction of response to therapy οƒ˜ Infections οƒ˜ In genetics οƒ˜ Neurodegenerative disorders οƒ˜ Brain trauma οƒ˜ IHC in muscle disease οƒ˜ Research application Application
  • 6. Polyclonal antibodies result in greater staining and excellent signal, but can give false positives by binding unwanted sites. Polyclonal Antibodies Monoclonal antibodies have a high specificity, reducing the number of false positive bindings, but often hive a much weaker stain. Monoclonal Antibodies Pooled monoclonal antibodies also give excellent staining and high specificity however there is limited availability for those do not bind noncompetitively. Pooled Monoclonal Antibodies Secondary antibodies, against the species of primary antibodies, will be labeled with an enzyme like HRP or biotin conjugated for staining or amplifying signal. Secondary Antibodies Selecting Antibodies
  • 7. IHC Methods Direct method PAP method LSAB method Methods ABC method Indirect method
  • 8. Methods β€’ One step staining method β€’ Labeled antibodies react directly with the antigen β€’ This method utilizes only one antibody and the procedure is short and quick β€’ It is insensitive due to little signal amplification and rarely used since the introduction of indirect method Direct Method Primary Antibody
  • 9. Methods β€’ An unlabeled primary antibody reacts with tissue antigen β€’ A labeled secondary antibody reacts with primary antibody β€’ More sensitive due to signal amplification through several secondary antibody reactions β€’ Economy since one labeled secondary antibody can be used with many primary antibodies β€’ The secondary antibody may be labeled with enzymes or fluorescent dyes Indirect Method Primary Antibody Secondary Antibody
  • 10. Methods β€’ A further development of the indirect method β€’ Involves a third layer which is a rabbit antibody to peroxidase. β€’ Bound to the unconjugated goat anti- rabbit gaba-globulin of the second layer. β€’ The sensitivity is about 100 to 1000 times higher β€’ Allows for much higher dilution of the primary antibody PAP Method Primary Antibody Secondary Antibody PAP Complex
  • 11. Methods β€’ A standard IHC method β€’ The technique involves three layers. β€’ The first layer is unlabeled primary antibody. The second layer is biotinylated secondary antibody. The third layer is a complex of avidin-biotin peroxidase. β€’ The peroxidase is then developed by the DAB or other substrate to produce different colorimetric end products. ABC Method Primary Antibody Biotinylated Secondary Antibody Avidin-biotin Peroxidase Complex
  • 12. Methods β€’ LSAB is similar to standard ABC method. β€’ The third layer is Enzyme-Streptavidin conjugates (HRP-Streptavidin or AP- Streptavidin) to replace the complex of avidin-biotin peroxidase. β€’ The third layer can also be Fluorescent dye-Streptavidin such as FITC- Streptavidin. β€’ Streptavidin does not contain carbohydrate groups which might bind to tissue lectins, avoiding some background staining. LSAB Method Primary Antibody Biotinylated Secondary Antibody Enzyme-Streptavidin Conjugates
  • 13. Protocol οƒ˜ Dip slides in three changes of xylene for 3 minutes each. οƒ˜ Dip slides in two change of 100% alcohol for 3 minutes each. οƒ˜ Dip slides in one change of 95% alcohol for 3 minutes. οƒ˜ Dip slides in one change of 70% alcohol for 3 minutes. οƒ˜ Rinse slides twice in dH2O for 5 minutes. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Deparaffinization & Rehydration
  • 14. Protocol οƒ˜ Soak slides in 3% H2O2 for 5 minutes. οƒ˜ Rinse slides twice in dH2O for 5 minutes. οƒ˜ Soak the slides in the working citrate buffer and cover with a lid. οƒ˜ Microwave until the liquid boils. οƒ˜ Remove from heat and let it stand at room temperature for 20 minutes. οƒ˜ Wash three times for 5 minutes in dH2O οƒ˜ Remove the liquid and use a PAP pen to circle around the tissue. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Antigen Retrieval
  • 15. Protocol οƒ˜ Apply enough 5% BSA with a transfer pipette to cover the tissues. οƒ˜ Incubate the slides overnight at 4℃ in a humid chamber. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Bloocking
  • 16. Protocol οƒ˜ Dilute the primary antibody to the recommended concentration in 1% BSA/PBS diluent. οƒ˜ Remove the BSA, and incubate with primary antibody solution for 1 hour at room temperature. οƒ˜ Wash slides three times 5 minutes each on the shaker. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Primary Antibody
  • 17. Protocol οƒ˜ Dilute the biotinylated secondary antibody in 1% BSA diluent. οƒ˜ Incubate with secondary antibody solution for 30 minutes at room temperature. οƒ˜ Wash slides in PBS three times, 5 minutes each on the shaker. οƒ˜ Add enough streptavidin HRP to cover the tissues. Incubate for 30 minutes at room temperature. οƒ˜ Wash three times 5 minutes each in PBS on the shaker. οƒ˜ Add enough DAB to cover the tissues. Once the cells start turning brown, wash twice in PBS for 5 minutes each on the shaker. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Secondary Antibody
  • 18. Protocol οƒ˜ Dip the slide rack with the slides into a staining dish of hematoxylin for 30 seconds. οƒ˜ Dip into an acetic bath (200mL dH2O with one to three drops of acetic acid). Rinse with dH2O. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Counterstain
  • 19. Protocol οƒ˜ Dip slides in 70% and 95% alcohol for 3 minutes each. οƒ˜ Dip slides in 2 changes of 100% alcohol for 3 minutes. οƒ˜ Dip slides in 3 changes of xylene or xylene substitute for 3 minutes. Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain Cover Slips Dehydration
  • 20. Protocol Deparaffinization & Rehydration Antigen Retrieval Blocking Primary Antibody Secondary Antibody Dehydration Counterstain οƒ˜ Apply coverslip to slide. οƒ˜ Let the slides dry overnight. Cover Slips Cover Slips
  • 21.