Immunohistochemical (IHC) Detection of Natural Cytotoxic Cells in Fish

Kathryn G. Smith; Matthew A. Sand; Niraj K. Tripathi, BVScAH; Louri J. Caldwell, HTL (ASCP); Donald L. Evans, PhD; and Kenneth S. Latimer, DVM, PhD

Undergraduate Honors Biology Program (Smith) and Undergraduate, Honors Microbiology Program (Sand), The University of Georgia, Athens, GA 30602; Department of Pathology (Tripahti, Caldwell, Latimer) and Department of Medical Microbiology and Parasitology (Evans), College of Veterinary Medicine, The University of Georgia, Athens, GA 30602

With the evolution of multicellular organisms, differentiated cells developed to protect these organisms against pathogens.  These differentiated cells provided the basis of immunity. More complex organisms, such as human beings, have a more intricate immune system. Therefore, comparative studies of less complex organisms provide additional information on immune system development and function. Basic knowledge and understanding of the of the human immune system have come from this kind of comparative research.¹  

One of the most basic understandings of immunity is that it provides a two-part defense system; humoral immunity and cell-mediated immunity.   Humoral immunity involves the production of antibodies against nonself antigens. Cell-mediated immunity requires viable effector cells that present antigens and destroy transformed or infected cells. Natural cytotoxic cells, like cytotoxic T-lymphocytes, seek and destroy transformed or infected cells. However, natural cytotoxic cells recognize and destroy their targets without the need for specific antigen presentation (this is in contrast to cytotoxic T-lymphocytes that require specific antigen presentation to recognize target cells).³  Thus, natural cytotoxic cells are essential for functional cell-mediated immunity and provide one of the first lines of defense to eliminate transformed or infected cells. 

The present study was done to determine whether immunohistochemistry (IHC) could identify natural cytotoxic cells in formalin fixed, paraffin embedded tissue sections of freshwater and marine fish. The ultimate goals of this study are to identify and quantitate natural cytotoxic cells in fish tissues and to determine if this cell population has a seasonal fluctuation that may affect overall immunity.

Fresh tissue specimens of an ornamental Koi (Cyprinus carpio) and black sea bass (Centropristis striata) were obtained and fixed in 10% neutral-buffered formalin solution. Formalin fixation did not exceed 24 hours (Figs. 1 & 2). The tissues were processed routinely, embedded in paraffin wax, and sectioned at 4 µm. Hematoxylin and eosin-stained slides were reviewed and sections of anterior (head) kidney and spleen were selected for IHC staining.²  Replicate tissue sections were cut for IHC, dewaxed, rehydrated through graded alcohols to buffer, and subjected to steam treatment to promote antigen retrieval. The primary antibody, designated 5C6, is a monoclonal IgM antibody that has been shown to specifically recognize natural cytotoxic cells in the blood of fish via flow cytometry (Fig. 3).³ This primary antibody was applied at a 1:10 dilution. Appropriate incubation was allowed for primary antibody attachment to the targeted site.  Following a brief wash in buffer solution, a secondary biotinylated antibody was added. After appropriate incubation and washing the avidin-biotin peroxidase complex was applied. A chromagen solution of 3,3’-diaminobenzidine tetrahydrochloride was used (Fig. 4). Following chromagen development, the sections were stained briefly in Gill’s hematoxylin, dehydrated through graded alcohols to xylene, coverslipped, and examined microscopically. Sites of primary antibody attachment were identified by the presence of an insoluble brown reaction product.

Fig. 1. Ornamental Koi (Cyprinus carpio), a freshwater member of the carp family.	Fig. 2. Black sea bass (Centropristis striata), a marine fish that can be raised commercially by mariculture techniques.

Fig. 3. Representation of an IgM antibody composed of a pentameric ring structure linked by disulfide bridges and a "J" chain. Courtesy of DAKO Corporation, Carpenteria, CA.	Fig. 4. Schematic of immunohistochemical staining using the avidin-biotin complex (ABC) technique. Courtesy of DAKO Corporation, Carpenteria, CA.

Piscine natural cytotoxic cells were readily indentified in sections of anterior kidney and spleen following IHC (Fig. 5 & 6). While the human implications of this research are mostly evolutionary, the ability to study populations of natural cytotoxic cells will facilitate research on the health and immunity of fish, a necessity for sustaining and advancing both aquaculture and mariculture.

Fig. 5. Histologic sections of anterior kidney demonstrating identification of natural cytotoxic cells following immunohistochemical staining. A. Hematoxylin and eosin-stained tissue section. B. Natural cytotoxic cells stain brown; ABC immunoperoxidase technique with DAB chromagen and Gill’s hematoxylin counterstain.

Fig. 6. Histologic sections of spleen demonstrating identification of natural cytotoxic cells following immunohistochemical staining. A. Hematoxylin and eosin-stained tissue section. B. Natural cytotoxic cells stain brown; ABC immunoperoxidase technique with DAB chromagen and Gill’s hematoxylin counterstain.

References

1. Pastoret PP, Griebel P, Bazin H, Govaerts A (eds): Handbook of Vertebrate Immunology, Academic Press, San Diego, CA, 1998.

2. Naish S, Boenisch T, Farmilo AJ, Stead RH: Handbook of Immunochemical Staining Methods, DAKO Corporation, Carpinteria, CA, 1989.

3. Jaso-Friedmann L, Evans DL, Grant CC, St John A, Harris DT, Koren HS: Characterization by monoclonal antibodies of a target cell antigen complex recognized by nonspecific cytotoxic cells. J Immunol 141:2861-2868, 1988.

^  Top of page