Summary
A recently developed immunocytochemical double-staining method for ultrathin Epon and Lowicryl K4M sections has been adopted for use on ultrathin cryosections. The essential features of the method include: staining for the first antigen by the indirect method using sufficient concentrations of second antibodies conjugated to colloidal gold particles to saturate available epitopes on the primary antibodies; supporting the cryosections by methyl cellulose followed by paraformaldehyde vapour treatment (30–60 min at 80°C); removal of the methyl cellulose followed by staining for the second antigen using primary antiserum from the same species and another size class of colloidal gold particles conjugated to second antibodies. Contaminating staining does not occur if the paraformaldehyde vapour treatment exceeds 30 min, as this treatment destroys the combining sites on the second antibodies applied in the first staining cycle. Succesful double-staining was documented using primary rabbit antibodies to growth hormone and corticotropin and anti-rabbit IgG conjugated to 5 and 15 nm colloidal gold particles. Following double-staining, the ultrathin cryosections may be silver-enhanced to improve detectability of the markers at low magnification.
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References
Bastholm L, Scopsi L, Nielsen MH (1986) Silver-enhanced immunogold staining of semithin and ultrathin cryosections. J Electron Microsc Tech 4:175–176
Bendayan M, Stephens H (1984) Double labelling cytochemistry applying the protein A gold technique. In: Polak JM, Varndell IM (eds) Immunolabelling for electron microscopy. Elsevier North-Holland, Amsterdam, pp 143–154
Geuze HJ, Slot JW, Scheffer RCT, van der Ley PA (1981) Use of colloidal gold particles in double-labelling immuno-electron microscopy of ultrathin frozen sections. J Cell Biol 89:653–665
Griffiths G, McDowell A, Back R, Dubochet J (1984) On the precipitation of cryosections for immunocytochemistry. J Ultrastruct Res 89:65–84
Slot JW, Geuze HJ (1984) Gold markers for single and double immunolabelling of ultrathin cryosections. In: Polak JM, Varndell IM (eds) Immunolabelling for electron microscopy. Elsevier North-Holland, Amsterdam, pp 129–142
Tokuyasu KT (1973) A technique for ultracryotomy of cell suspensions and tissues. J Cell Biol 57:551–565
Tokuyasu KT (1978) A study of positive staining of ultrathin frozen sections. J Ultrastruct Res 63:287–307
Varndell IM, Polak JM (1984) Double immunostaining procedures: Techniques and applications. In: Polak JM, Varndell IM (eds) Immunolabelling for electron microscopy. Elsevier North-Holland, Amsterdam, pp 155–177
Wang B-L, Larsson L-I (1985) Simultaneous demonstration of multiple antigens by direct immunofluorescense or immunogold staining. Novel light and electron microscopical double and triple staining method employing primary antibodies from the same species. Histochemistry 83:47–56
Young WW, Tamura Y, Wolock DM, Fox JW (1984) Staphylococcal protein A binding to the Fab fragments of mouse monoclonal antibodies. J Immunol 133:3163–3166
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Bastholm, L., Nielsen, M.H. & Larsson, L.I. Simultaneous demonstration of two antigens in ultrathin cryosections by a novel application of an immunogold staining method using primary antibodies from the same species. Histochemistry 87, 229–231 (1987). https://doi.org/10.1007/BF00492414
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DOI: https://doi.org/10.1007/BF00492414