口腔免疫的靶向策略——大鼠M细胞标记抗原的鉴定。

Behring Institute Mitteilungen Pub Date : 1997-02-01
K Rautenberg, C Cichon, M A Schmidt
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引用次数: 0

摘要

胃肠道和呼吸道Peyer's斑块的滤泡相关上皮(FAE)的特化M细胞在粘膜表面的免疫监视中起着至关重要的作用,并且对诱导粘膜免疫反应至关重要。这些细胞将腔内抗原运送到潜在的生发中心,从而启动免疫反应或诱导耐受。口服抗原直接靶向M细胞的根尖表面,可显著增强粘膜免疫应答。然而,到目前为止,M细胞还没有被分离出来,合适的表面标记物也没有被描述。为了鉴定M细胞的潜在分子标志物,采用间接免疫荧光和免疫金电镜对大鼠小肠Peyer’s patches的卵泡相关上皮进行了分析。发现FAE中中间丝蛋白的表达具有异质性。特异性单克隆细胞角蛋白8抗体(克隆为4.1.18)在细胞中选择性地发现了免疫反应性,另外,在细胞的顶膜中缺乏碱性磷酸酶染色。在FAE中,这一特性是M细胞存在的公认标准。与邻近的上皮细胞或“正常”肠细胞相比,克隆4.1.18识别的抗原在Peyer’s patches M细胞中的表达量要高得多,因此可以作为大鼠Peyer’s patches M细胞的细胞内分子标记物。预计该标记物将对M细胞的分离有很大的帮助。
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Towards targeting strategies for oral immunization--identification of marker antigens in rat M cells.

Specialized M cells of the follicle-associated epithelium (FAE) of Peyer's patches in the gastrointestinal and respiratory tracts play a crucial role in the immune surveillance of mucosal surfaces and are essential for the induction of mucosal immune responses. These cells transport luminal antigens to the underlying germinal centers and thereby initiate an immune response or induce tolerance. Mucosal immune responses could be significantly enhanced if oral antigens could be directly targeted to the apical surface of M cells. However, thus far M cells have not been isolated and suitable surface markers have not been described. For the characterization and identification of potential molecular markers of M cells the follicle associated epithelium of Peyer's patches from the small intestine of rats was analyzed by indirect immunofluorescence and immunogold electronmicroscopy. The expression of intermediate filament proteins in the FAE was found to be heterogeneous. Immunoreactivity of a specific monoclonal cytokeratin 8 antibody (clone 4.1.18) was selectively found in cells which were additionally characterized by the lack of staining for alkaline phosphatase in their apical membranes. In the FAE this property is an accepted criterium for the presence of M cells. The antigen recognized by the clone 4.1.18 is expressed in substantially higher amounts in M cells of Peyer's patches as compared to neighbouring epithelial cells or "normal" enterocytes and thus can be employed as an intracellular molecular marker for M cells of Peyer's patches in rats. It is expected, that this marker will be very helpful for the isolation of M cells.

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