Recent publications indicate that interleukin

(IL) T help

Recent publications indicate that interleukin

(IL) T helper type 9 (Th9) cells play an important role in immune inflammation [5,6]. Th9 cells express IL-9 that increases IL-4-induced immunoglobulin (Ig)E production [7], activates Apoptosis Compound Library in vitro mast cells [8] and enhances production of chemokines [7]. A subset of T cells, IL-9+ IL-10+ T cells, which have been described recently, is involved in the induction of immune inflammation [9]. The source of this subset of T cells in the body is unknown. As both IL-9 and IL-10 belong to T helper type 2 (Th2) cytokines, IL-9+ IL-10+ T cells may be involved in the pathogenesis of allergy. Exposure to IL-9+ IL-10+ T cells can induce profound inflammation in the intestine that featured as abundant inflammatory cell extravasation in local tissue [9]. Such inflammation characterized as excessive inflammatory cell extravasation does not usually occur in immediate allergic reactions, but more probably occurs in LPR. Thus, we hypothesize that IL-9+ IL-10+ T cells play an important role in the pathogenesis of LPR. By employing the intestine selleck compound as a study platform, we developed a Th2 inflammation mouse model to dissect the role of IL-9+ IL-10+ T cell in the pathogenesis of LPR. Indeed, the results showed that IL-9+ IL-10+ T cells were involved in the specific antigen-induced LPR. Activation of the IL-9+ IL-10+ T cells

contributed to the inflammatory cell extravasation in the intestine. The data imply that this subset of CD4+ T cell has the potential to be a novel therapeutic target in the treatment of LPR. BALB/c mice, 6–8 weeks old, were purchased from Charles River Canada (St Constant, QC, Canada). Ovalbumin-T cell receptor (OVA-TCR) transgenic mice were purchased from Jackson Laboratory (Bar Harbor, MI, USA). The procedures of animal experiments in this study were approved by the Animal Care Committee at

McMaster University. Verteporfin datasheet The procedures to establish a Th2 polarization mouse model were depicted in Fig. 1a. Parameters of intestinal Th2 inflammation were examined with our established procedures that included: levels of serum OVA-specific IgE antibody, serum histamine, numbers of mast cells, eosinophils and mononuclear cells in the lamina propria and antigen-specific Th2 cell proliferation. Segments of the intestine were fixed with 4% paraformaldehyde overnight and processed for paraffin embedding. Sections were stained with haematoxylin and eosin. Tissue structure was observed under a light microscope by a staff pathologist who was unaware of the treatment. Mononuclear cells, eosinophils, neutrophils and mast cells were numerated at a magnification of ×200; 30 fields/mouse (for mast cell counting, tissue was fixed with Carnoy solution; sections were stained with 0·5% toluidine blue).

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