Triple Immunofluorescence Staining with Antibodies Raised in the Same Species to Study the Complex Innervation Pattern of Intrapulmonary Chemoreceptors

Journal of Histochemistry and Cytochemistry

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Triple Immunofluorescence Staining with Antibodies Raised in the Same Species to Study the Complex Innervation Pattern of Intrapulmonary Chemoreceptors

Inge Brouns^a, Luc Van Nassauw^a, Jeroen Van Genechten^a, Mariusz Majewski^b, Dietrich W. Scheuermann^a, Jean-Pierre Timmermans^a, and Dirk Adriaensen^a
^a Laboratory of Cell Biology and Histology, University of Antwerp (RUCA), Antwerp, Belgium
^b Department of Clinical Physiology, Warmia and Mazury University, Olsztyn, Poland

Correspondence to: Dirk Adriaensen, Laboratory for Cell Biology & Histology, University of Antwerp, Groenenborgerlaan 171, B-2020 Antwerp, Belgium. E-mail: dadria@ruca.ua.ac.be

A general problem in immunocytochemistry is the developmentof a reliable multiple immunolabeling method when primary antibodiesmust be used that originate in the same species. We have developeda protocol for the immunodetection of three antigens in a singletissue preparation, using unconjugated primary antibodies raisedin the same species. Immunocytochemical detection of neuronalnitric oxide synthase, calcitonin gene-related peptide, andcalbindin D28k in the lung of rats demonstrated that part ofthe pulmonary neuroepithelial bodies are selectively contactedby at least three different nerve fiber populations. The firstantigen was detected using tyramide signal amplification, avery sensitive method allowing a dilution of the first primaryantibody far beyond the detection limit of fluorescently labeledsecondary antibodies. The second antigen was visualized by afluorophore-conjugated secondary monovalent Fab antibody thatat the same time blocks the access of the third secondary antibodyto the second primary antibody. Moreover, the monovalence ofthe Fab fragment prevents the third primary antibody from bindingwith the second-step secondary antibody. The triple stainingtechnique described here is generally applicable, uses commerciallyavailable products only, and allows the detection of three antigensin the same preparation with primary antibodies that are raisedin the same species. (J Histochem Cytochem 50:575–582,2002)

Key Words: triple immunostaining, multiple immunostaining, same species,tyramide signal amplification, Fab secondary antibodies, pulmonaryneuroepithelial, bodies, confocal laser scanning, microscopy

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