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W tym Artykule

  • Podsumowanie
  • Streszczenie
  • Wprowadzenie
  • Protokół
  • Wyniki
  • Dyskusje
  • Ujawnienia
  • Podziękowania
  • Materiały
  • Odniesienia
  • Przedruki i uprawnienia

Podsumowanie

Several different methods have been established for multiplex immunostaining using primary antibodies from the same host species. Here, we describe the use of microwave-mediated antibody stripping and of fluorophore-tyramide to block antibody cross-reactivity during multiplex immunostaining on formalin-fixed paraffin-embedded mouse adrenal sections.

Streszczenie

Immunostaining is widely used in biomedical research to show the cellular expression pattern of a given protein. Multiplex immunostaining allows labeling using multiple primary antibodies. To minimize antibody cross-reactivity, multiplex immunostaining using indirect staining requires unlabeled primary antibodies from different host species. However, the appropriate combination of different species antibodies is not always available. Here, we describe a method of using unlabeled primary antibodies from the same host species (e.g., in this case both antibodies are from rabbit) for multiplex immunofluorescence on formalin-fixed paraffin-embedded (FFPE) mouse adrenal sections. This method uses the same procedure and reagents used in the antigen retrieval step to strip the activity of the previously stained primary antibody complex. Slides were stained with the first primary antibody using a general immunostaining protocol followed by a binding step with a biotinylated secondary antibody. Then, an avidin-biotin-peroxidase signal development method was used with fluorophore-tyramide as the substrate. The immunoactivity of the first primary antibody complex was stripped through immersion in a microwaved boiling sodium citrate solution for 8 min. The insoluble fluorophore-tyramide deposition remained on the sample, which allowed the slide to be stained with other primary antibodies. Although this method eliminates most false positive signals, some background from antibody cross-reactivity may remain. If the samples are enriched with endogenous biotin, a peroxidase-conjugated secondary antibody may be used to replace the biotinylated secondary antibody to avoid the false positive from recovered endogenous biotin.

Wprowadzenie

In multiplex immunostaining, direct staining using conjugated primary antibodies can provide informative results. Without using secondary antibodies, the direct staining method has a low risk of false colocalization signals from antibody cross-reactivity. However, the conjugated reporters (fluorophore, enzymes) or biotin on the primary antibody limit its future use. Alternatively, indirect immunostaining usually provides stronger signals by using an unconjugated primary antibody with a labeled secondary antibody. Ideally, unconjugated primary antibodies used in multiplex immunostaining should come from different host species to avoid antibody cross-reactivity. However, the appropriate combination of primary antibodies from different host species is not always available.

Several methods have been established to eliminate the risk of the secondary antibody reacting with an undesired primary antibody. One common method is the use of a F(ab) monomeric antibody to block any remaining binding epitopes on the first primary antibody complex before staining with the second primary antibody1. Antibody stripping, which is similar to the strip and reprobe of a Western blot sheet, removes the previously stained antibody complex without stripping the deposition of detectable reporter molecules such as 3,3'-diaminobenzidine tetrahydrochloride (DAB)2 and the fluorescent tyramide deposition3. With this method, reporter molecules in different colors can show a multiplex result on the same slide. The multiplex staining is also achievable by the complete removal of the previously deposited layers of antibodies and the alignment of subsequently acquired images from other antibodies4,5. These methods all give reliable results, though each method has its limitations and requires either complicated procedures or a special imaging system.

The present protocol shows the application of an antibody stripping method with the use of commonly available buffers. This protocol can be used to perform multiplex immunofluorescent staining on formalin-fixed paraffin-embedded (FFPE) mouse adrenal sections with two unlabeled primary antibodies from the same host species.

Protokół

1. Staining with the First Antibody

  1. Dewax and rehydrate FFPE slides with 5 min allotted to each of the following steps: xylene or equivalent reagents 3x, 100% ethanol 2x, 95% ethanol 1x, 70% ethanol 1x, 50% ethanol 1x, and distilled water 2x.
    NOTE: Slides should remain moist starting from this rehydration step until mounting in the final step.
  2. For optional antigen retrieval, place the slides in 275 mL of boiling sodium citrate solution (10 mM, pH = 6.0) for 8 min. To keep the solution boiling, place the slides flat on the bottom of a 14 x 9.5 x 9 cm3 (W x L x H) pipette tip box with a lid and microwave the solution on 70% power in a 700 W microwave oven for 8 min. Then remove the pipette tip box from the microwave oven, open the lid, and let the solution cool down at room temperature (RT) for at least 20 min.
  3. Transfer the slides into a Coplin jar containing PBST (phosphate-buffered saline with 0.1% polysorbate 20/80). Wash with PBST for 5 min 3x. If not immediately moving to the next step, store the slides at this step with PBST in a Coplin jar at RT for a few hours or at 4 °C for 1-2 days if not immediately moving to the next step.
  4. To prepare the blocking solution use the normal serum of the secondary antibody's host species as the blocking reagent. Other commercial blocking reagents may also be used. If using normal serum employed for the study presented in this study, add 100 µL of normal donkey serum to 4.9 mL of PBST. The blocking solution can be stored at 4 °C for up to 3 days.
  5. For blocking, shake off the PBST from the slides and quickly cover them with sufficient blocking solution. Incubate the slides at RT in a humidified chamber for 30 min.
  6. Prepare the primary antibody solution (500 µL for two slides) using the blocking solution to dilute the primary antibody to the desired concentration. The solution should be stored on ice until use.
    1. For 3βHSD, add 2 µL of 3βHSD into 498 µL of blocking solution.
    2. For TH, add 0.5 µL of TH antibody into 499 µL of blocking solution.
    3. For β-catenin, add 1 µL of β-catenin antibody into 499 µL of blocking solution.
    4. For 20αHSD, add 1 µL of 20αHSD antibody into 499 µL of blocking solution.
    5. For CYP2F2, add 2 µL of CYP2F2 antibody into 498 µL of blocking solution.
  7. Incubate with the primary antibody by shaking off the blocking solution from the slides, and quickly covering them with sufficient primary antibody solution. Incubate the slides in a humidified chamber overnight at 4 °C. During incubation the slides may be covered by a small piece of paraffin film to prevent drying out.
  8. The next morning wash the slides with PBST for 5 min 3x.
  9. Prepare the secondary antibody solution (500 µL for two slides) using the blocking solution to dilute the biotinylated secondary antibody to the desired concentration (e.g., 1 µL of donkey anti-mouse antibody or donkey anti-rabbit antibody into 499 µL of blocking solution). The solution should be stored on ice until use.
  10. Incubate with the second antibody by shaking off PBST from the slides and quickly covering them with sufficient secondary antibody solution. Incubate the slides in a humidified chamber for 1 h at RT.
    NOTE: If endogenous biotin is a concern, use a peroxidase-conjugated secondary antibody instead of the biotinylated secondary antibody. Jump to step 1.14 if using a peroxidase-conjugated secondary antibody in step 1.10.
  11. Wash the slides with PBST for 5 min 3x.
  12. Prepare the horseradish peroxidase-conjugated streptavidin (SA-HRP) solution (500 µL for two slides) by adding 0.5 µL of SA-HRP into 499 µL of PBS. The final concentration is 1 µg/mL.
  13. Incubate with the SA-HRP solution. Shake off PBST from the slides and quickly cover the slides with sufficient SA-HRP solution. Incubate the slides in a humidified chamber for 0.5 h at RT.
  14. Wash the slides with PBST for 5 min 3x.
  15. Prepare the fluorophore-tyramide solution by diluting fluorophore-tyramide with its dilution buffer according to the manufacturer's instructions (e.g., 5 µL of fluorophore-tyramide into 496 µL of dilution buffer).
  16. Perform the signal development with fluorophore-tyramide by shaking off PBST from the slides and quickly covering the slides with sufficient fluorophore-tyramide solution. Incubate in a humidified chamber for 1 min at RT. The incubation time may be adjusted to obtain the desired fluorescence intensity. Stop the reaction by transferring the slides to a Coplin jar containing PBST. Wash slides with PBST for 3 min 2x.
  17. Signals may be quickly checked under a fluorescence microscope to confirm the result at this stage. If coverslips are not being used, apply a drop of glycerol:PBS (1:1) onto each section to keep the samples moist. Wash slides with PBST for 3 min 2x. Slides may be stored in PBST at 4 °C for a few days before moving to the next step.

2. Strip the First Antibody

  1. Place the slides in 275 mL of boiling sodium citrate solution (10 mM, pH = 6.0) for at least 8 min. Keep the solution boiling by placing the slides flat on the bottom of a 14 x 9.5 x 9 cm3 (W x L x H) pipette tip box with a lid and microwaving the solution on 70% power in a 700 W microwave oven for 8 min. If a longer stripping time is preferred, it may be required to top off the buffer using a boiling sodium citrate solution to keep the slides immersed in buffer solution at all times. Remove the pipette tip box from the microwave oven, open the lid, and let the solution cool down at RT for at least 20 min.
  2. Transfer the slides into a Coplin jar containing PBST. Wash with PBST for 5 min 3x. If the next step if not performed immediately, store the slides in a Coplin jar with PBST at RT for a few hours or at 4 °C for 1-2 days.

3. Stain with the Second Antibody

  1. Start from the blocking step and follow same procedures in step 1.5 through step 1.14. At the signal development steps (step 1.15 and step 1.16), use the fluorophore-tyramide in a different fluorescence spectrum.
    NOTE: Slides can be stripped using this method several times to allow multiplex staining. The last antibody does not require fluorophore-tyramide as the reporter. A fluorophore-conjugated secondary antibody might be used to show signals from the last primary antibody.
  2. Incubate slides with 2 µg/mL 4',6-diamidino-2-phenylindole (DAPI) or Hoechst solution for 1 min at RT if nuclear counter staining is needed. Then wash the slides with PBST for 3 min 2x.

4. Imaging Using a Fluorescence Microscope to Detect Signals

  1. Mount a coverslip with a drop of mounting medium suitable for immunofluorescence.
  2. For imaging, use a fluorescence microscope to detect signals of each fluorescence channel. Start with the nuclear staining (DAPI) channel and the 4x lens to locate the tissue on the slide.
  3. Switch to the 10x lens for imaging. Adjust the exposure time (300 ms) and light source intensity (80% intensity). Adjust these settings if the signal is too bright or too dark. Take pictures of each channel without moving the stage. Refocusing may be needed for each channel. Merge the images from each channel using the microscope's software or ImageJ (imagej.nih.gov/ij/).

Wyniki

The results were obtained from samples treated with all steps described including the antigen retrieval step 1.2. All secondary antibodies used here were biotinylated. Fluorophore-tyramide was used to develop signals from the first and second primary antibodies. Images were captured using a fluorescence microscope equipped with a FITC cube (for green fluorescence), a TxRED cube (for Cy3), and a DAPI cube (for DAPI).

Micr...

Dyskusje

Multiplex immunostaining is useful to examine the cellular colocalization of two or more antigens. This widely used technique gives convincing colocalization results when primary antibodies are conjugated with different reporters (direct staining). However, direct staining usually provides weaker signals compared to indirect staining, which involves conjugated secondary antibodies to detect the primary antibodies. In indirect staining, a high-quality multiplex immunostaining result relies on whether the secondary antibod...

Ujawnienia

The authors have nothing to disclose.

Podziękowania

This work is supported by NIH R00 HD032636.

Materiały

NameCompanyCatalog NumberComments
Antifade Mounting MediumVector LaboratoriesH-1000
Biotinylated donkey anti-mouseJacksonImmuno715-066-1511:500 dilution
Biotinylated donkey anti-rabbitJacksonImmuno711-066-1521:500 dilution
DAPIBioLegend4228012 μg/mL in distilled water
Fluorescence microscopeECHORevolve 4
Horseradish peroxidase-conjugated streptavidinJacksonImmuno016-030-0841:1,000 dilution
Microwave oven, 700 WGeneral ElectricJEM3072DH1BB
Mouse anti-CYP2F2Santa CruzSC-3745401:250 dilution
Mouse anti-THSanta CruzSC-252691:1,000 dilution
Normal donkey serumJacksonImmuno017-000-1212% serum in PBST
Rabbit anti-20αHSDKerafastEB40021:500 dilution
Rabbit anti-3βHSDTransGenicKO6071:250 dilution
Rabbit anti-THNOVUSNB300-1091:1,000 dilution
Rabbit anti-β-cateninAbcamab325721:500 dilution
Streptavidin Horseradish Peroxidase (SA-HRP)JacksonImmuno016-303-0841:1,000 dilution
TSA Cy3 TyramidePerkinElmerSAT704B001EA1:100 dilution
TSA Fluorescein TyramidePerkinElmerSAT701001EA1:100 dilution

Odniesienia

  1. Lewis Carl, S. A., Gillete-Ferguson, I., Ferguson, D. G. An indirect immunofluorescence procedure for staining the same cryosection with two mouse monoclonal primary antibodies. Journal of Histochemistry and Cytochemistry. 41 (8), 1273-1278 (1993).
  2. Lan, H. Y., Mu, W., Nikolic-Paterson, D. J., Atkins, R. C. A novel, simple, reliable, and sensitive method for multiple immunoenzyme staining: use of microwave oven heating to block antibody crossreactivity and retrieve antigens. Journal of Histochemistry and Cytochemistry. 43 (1), 97-102 (1995).
  3. Tornehave, D., Hougaard, D. M., Larsson, L. Microwaving for double indirect immunofluorescence with primary antibodies from the same species and for staining of mouse tissues with mouse monoclonal antibodies. Histochemistry and Cell Biology. 113 (1), 19-23 (2000).
  4. Kim, M., Soontornniyomkij, V., Ji, B., Zhou, X. System-wide immunohistochemical analysis of protein co-localization. PLoS One. 7 (2), e32043 (2012).
  5. Bolognesi, M. M., et al. Multiplex Staining by Sequential Immunostaining and Antibody Removal on Routine Tissue Sections. Journal of Histochemistry and Cytochemistry. 65 (8), 431-444 (2017).
  6. Toth, Z. E., Mezey, E. Simultaneous visualization of multiple antigens with tyramide signal amplification using antibodies from the same species. Journal of Histochemistry and Cytochemistry. 55 (6), 545-554 (2007).
  7. Buchwalow, I., Samoilova, V., Boecker, W., Tiemann, M. Multiple immunolabeling with antibodies from the same host species in combination with tyramide signal amplification. Acta Histochemica. 120 (5), 405-411 (2018).
  8. Bauer, M., Schilling, N., Spanel-Borowski, K. Limitation of microwave treatment for double immunolabelling with antibodies of the same species and isotype. Histochemistry and Cell Biology. 116 (3), 227-232 (2001).
  9. Pirici, D., et al. Antibody elution method for multiple immunohistochemistry on primary antibodies raised in the same species and of the same subtype. Journal of Histochemistry and Cytochemistry. 57 (6), 567-575 (2009).
  10. Glass, G., Papin, J. A., Mandell, J. W. SIMPLE: a sequential immunoperoxidase labeling and erasing method. Journal of Histochemistry and Cytochemistry. 57 (10), 899-905 (2009).
  11. Zhang, W., et al. Fully automated 5-plex fluorescent immunohistochemistry with tyramide signal amplification and same species antibodies. Laboratory Investigation. 97 (7), 873-885 (2017).
  12. Paul, A., Laufer, E. Endogenous biotin as a marker of adrenocortical cells with steroidogenic potential. Molecular and Cellular Endocrinology. 336 (1-2), 133-140 (2011).
  13. Bussolati, G., Gugliotta, P., Volante, M., Pace, M., Papotti, M. Retrieved endogenous biotin: a novel marker and a potential pitfall in diagnostic immunohistochemistry. Histopathology. 31 (5), 400-407 (1997).
  14. Wang, H., Pevsner, J. Detection of endogenous biotin in various tissues: novel functions in the hippocampus and implications for its use in avidin-biotin technology. Cell and Tissue Research. 296 (3), 511-516 (1999).

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