Enhanced intestinal transepithelial antigen transport in allergic rats is mediated by IgE and CD23 (FcεRII)
Ping-Chang Yang, … , Daniel H. Conrad, Mary H. Perdue
Ping-Chang Yang, … , Daniel H. Conrad, Mary H. Perdue
Published October 1, 2000
Citation Information: J Clin Invest. 2000;106(7):879-886. https://doi.org/10.1172/JCI9258.
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Article

Enhanced intestinal transepithelial antigen transport in allergic rats is mediated by IgE and CD23 (FcεRII)

Abstract

We previously reported that active sensitization of rats resulted in the appearance of a unique system for rapid and specific antigen uptake across intestinal epithelial cells. The current studies used rats sensitized to horseradish peroxidase (HRP) to define the essential components of this antigen transport system. Sensitization of rats to HRP stimulated increased HRP uptake into enterocytes (significantly larger area of HRP-containing endosomes) and more rapid transcellular transport compared with rats sensitized to an irrelevant protein or naive control rats. Whole serum but not IgE-depleted serum from sensitized rats was able to transfer the enhanced antigen transport phenomenon. Immunohistochemistry demonstrated that sensitization induced expression of CD23, the low-affinity IgE receptor (FcεRII), on epithelial cells. The number of immunogold-labeled CD23 receptors on the enterocyte microvillous membrane was significantly increased in sensitized rats and was subsequently reduced after antigen challenge when CD23 and HRP were localized within the same endosomes. Finally, pretreatment of tissues with luminally added anti-CD23 antibody significantly inhibited both antigen transport and the hypersensitivity reaction. Our results provide evidence that IgE antibodies bound to low-affinity receptors on epithelial cells are responsible for the specific and rapid nature of this novel antigen transport system.

Authors

Ping-Chang Yang, M. Cecilia Berin, Linda C.H. Yu, Daniel H. Conrad, Mary H. Perdue

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Figure 1

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HRP uptake into enterocyte endosomes. HRP was added to the mucosal buffe...
HRP uptake into enterocyte endosomes. HRP was added to the mucosal buffer of chambers containing jejunal tissues obtained from naive control rats or rats actively sensitized to OVA or HRP. Tissues were fixed for electron microscopy 2 minutes after HRP challenge and processed to visualize HRP reaction product. Representative photomicrographs are shown for tissues obtained from: (a) a rat actively sensitized to HRP, (b) a rat passively sensitized to HRP, or (c) a naive control rat. HRP-containing endosomes are indicated by arrowheads (bars indicate 1 μm). These photomicrographs are representative of those used to obtain the quantitative measurements of endosomal area shown in (d). Upper panel: active sensitization. Rats, actively sensitized to OVA or HRP, were compared with naive controls (CON); jejunal tissues from all rats were challenged with HRP. The total area of HRP endosomes was measured in fixed-size windows in the apical region of enterocytes. Lower panel: passive sensitization. For passive sensitization, experimental rats were injected intraperitoneally with serum from actively sensitized rats, either untreated [IgE+], heat-treated [IgE– (heat)], or IgE-depleted [IgE– (i-ppt)]. Values represent means ± SEM. AP < 0.01 compared with control; n = 12–24 views analyzed for each group (from four rats per group).