Delineation of the healthy rabbit tonsil by immunohistochemistry - A short communication

Gabriella Meier Bürgisser; Dorothea M Heuberger; Pietro Giovanoli; Maurizio Calcagni; Johanna Buschmann

doi:10.1016/j.acthis.2023.152098

Delineation of the healthy rabbit tonsil by immunohistochemistry - A short communication

Acta Histochem. 2023 Oct;125(7):152098. doi: 10.1016/j.acthis.2023.152098. Epub 2023 Oct 5.

Authors

Gabriella Meier Bürgisser¹, Dorothea M Heuberger², Pietro Giovanoli¹, Maurizio Calcagni¹, Johanna Buschmann³

Affiliations

¹ Division of Plastic Surgery and Hand Surgery, University Hospital Zurich, Sternwartstrasse 14, 8091 Zurich, Switzerland.
² Institute of Intensive Care Medicine, University Hospital Zurich, Sternwartstrasse 14, 8091 Zurich, Switzerland.
³ Division of Plastic Surgery and Hand Surgery, University Hospital Zurich, Sternwartstrasse 14, 8091 Zurich, Switzerland. Electronic address: johanna.buschmann@usz.ch.

PMID: 37804548
DOI: 10.1016/j.acthis.2023.152098

Abstract

Situated in the oral cavity, the rabbit palatine tonsils are part of the mucosal immune system and help to defend the body against foreign pathogens. Expressed as two oval protrusions in the wall of the oropharynx, the rabbit palatine tonsils are characterized by excretory ducts and trabeculae. We here compare paraffin embedded and cryosections of the healthy rabbit tonsils. This analysis centers on evaluating the differential outcomes resulting from the application of these fixation methodologies in conjunction with immunohistochemical assays targeting collagen I, collagen III, fibronectin, α-smooth muscle actin (α-SMA), and ki67. Subsequent recommendations are provided based on our findings. Furthermore, we demonstrate the advantage of an antigen retrieval step in immunohistochemical labeling of paraffin sections. Basic classical histological stainings as HE, GT and elastin were also performed. Comparison of different stainings and labelings was furthermore performed in serial sections, showing that adjacent to the excretory ducts, the tonsillar tissue was particularly composed of collagen I and fibronectin, while the vessel walls were predominantly α-SMA positive. Moreover, PAR-2 immunohistochemical staining was performed, where a small fraction of the cells found in the tonsillar connective tissue were PAR-2 positive (probably a subpopulation of mast cells), as well as the lumen of some excretory ducts and trabeculae. Collagen III on the other hand was only weakly expressed in the tonsils. Proliferating ki67 positive cells were rare. This endeavor serves to furnish the scientific community with reference imagery pertinent to researchers opting for the rabbit palatine tonsil model. The diversity of staining techniques employed herein establishes a foundational repository of images, primed for comparative analysis against pathological conditions. Furthermore, these images hold the potential to illustrate inter-species variations. For instance, they can be juxtaposed against murine or rodent tonsils, or even offer insights into the human context.

Keywords: Antigen retrieval; Cryosection; Excretory duct; Immunofluorescence; Trabeculae.

MeSH terms

Animals
Collagen
Fibronectins*
Humans
Immunohistochemistry
Ki-67 Antigen
Mice
Palatine Tonsil* / chemistry
Paraffin / analysis
Rabbits

Substances

Fibronectins
Ki-67 Antigen
Paraffin
Collagen