The IHC-plus Immunohistochemistry Protocol
LSBio has tested and validated monoclonal antibodies (mouse, rabbit, rat), polyclonal antibodies (rabbit, goat, sheep, llama, chicken), and human
single and double chain antibodies for use in immunohistochemistry (IHC) using formalin-fixed paraffin-embedded tissues, the most common fixation
method used by pathology labs worldwide. After 15 years of experience performing contract IHC research, creating immunohistochemistry localization
databases, and producing and testing antibodies in IHC, we have acquired a substantial body of experience regarding IHC and what protocol works
with the highest percentage of commercial antibodies and available tissues. The following summarizes our protocol and approach toward IHC antibody
validation.
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Tissue Preparation
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- Formalin fixation and embedding in paraffin wax
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Tissue Sectioning
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- Make 4-µm sections and place on pre-cleaned and charged microscope slides.
- Heat in a tissue-drying oven for 45 minutes at 60°C
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Deparaffinization
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- Wash slides in 3 changes of xylene – 5 minutes each @ RT
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Rehydration
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- Wash slides in 3 changes of 100% alcohol – 3 minutes each @ RT
- Wash slides in 2 changes of 95% alcohol – 3 minutes each @ RT
- Wash slides in 1 change of 80% alcohol – 3 minutes @ RT
- Rinse slides in gentle running distilled water – 5 minutes @ RT
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Antigen retrieval
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- Steam slides in 0.01 M sodium citrate buffer, pH 6.0 at 99-100°C - 20 minutes
- Remove from heat and let stand at room temperature in buffer - 20 minutes
- Rinse in 1X TBS with Tween (TBST) – 1 minute @ RT
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Immunostaining
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- Do not allow tissues to dry at any time during the staining procedure.
- Apply a universal protein block – 20 minutes @ RT
- Drain protein block from slides, apply diluted primary antibody – 45 minutes @ RT
- Rinse slides in 1X TBST - 1 minute @ RT
- Apply alkaline phosphatase streptavidin – 30 minutes @ RT
- Rinse slides in 1X TBST - 1 minute @ RT
- Apply alkaline phosphatase chromogen substrate – 30 minutes @ RT
- Wash slides in distilled water – 1 minute @ RT
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Dehydrate
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- This method should only be used if the chromogen substrate is alcohol insoluble.
- Wash slides in 2 changes of 80% alcohol – 1 minute each @ RT
- Wash slides in 2 changes of 95% alcohol – 1 minute each @ RT
- Wash slides in 3 changes of 100% alcohol – 1 minute each @ RT
- Wash slides in 3 changes of xylene – 1 minute each @ RT
- Apply coverslip
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LSBio's IHC-plus antibodies
have been tested and identified as being optimal for use in immunohistochemistry (IHC) against formalin-fixed paraffin-embedded (FFPE)
human tissues under LSBio's standardized IHC-plus protocol. Each antibody is tested at multiple concentrations on more than 20
normal human tissue types, and when appropriate, multiple normal brain regions and/or cancer types. LSBio's IHC protocol has been developed
over the past 15 years as the most optimal method of immunolabeling FFPE tissues, the most common fixation method used by pathology
labs worldwide. A LifeSpan pathologist, with extensive experience evaluating IHC, analyzes the localization profile of each antibody,
identifying positive and negative cell types, signal strength, subcellular and extracellular staining, and staining artifacts. This
information is then compared with all published expression and localization data available for the protein. This enables LSBio to evaluate
how each antibody behaves in IHC, including its specificity to the target protein, its sensitivity of detection, and any non-specific
staining characteristics that it may display. In order to be selected as an IHC-plus brand antibody, antibodies must have a close
correlation to the published literature, be high affinity, display minimal staining artifacts, and have a high signal-to-noise ratio, such
that its specific staining is considerably higher than its level of nonspecific background staining. Only the best antibodies receive approval
and are given the designation as LSBio's premier IHC-plus antibodies.
Learn more about LSBio's Immunohistochemistry (IHC) Validation
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