Rossi G A, Sacco O, Balbi B, Oddera S, Mattioni T, Corte G, Ravazzoni C, Allegra L
I. Divisione di Pneumologia, Ospedale San Martino, Genoa, Italy.
Am J Respir Cell Mol Biol. 1990 Nov;3(5):431-9. doi: 10.1165/ajrcmb/3.5.431.
HLA-DR class II molecules are expressed by a variety of nonlymphoid cells, including the respiratory epithelium. However, it is not known if ciliated bronchial epithelial cells express the HLA-DR genes, if the expression of class II molecules on their surface can be modulated by immune mediators and, finally, if these cells, like other HLA-DR-positive epithelial cells, have the potential to serve as antigen-presenting cells. To answer these questions, we collected ciliated bronchial epithelial cells by brushing and by suction during fiberoptic bronchoscopy and by scraping surgically resected bronchi. The number of cells recovered by brushing or suction during fiberoptic bronchoscopy was similar (P greater than 0.2), but lower than that obtained by scraping surgically resected bronchi (P less than 0.01); however, compared with brushing, suction of ciliated bronchial epithelial cells resulted in a better viability (P less than 0.05). HLA-DR antigens on ciliated bronchial epithelial cells were detected by immunofluorescence using the PTF 29.12 and the L243 monoclonal antibodies, both recognizing HLA-DR molecules on the vast majority of ciliated bronchial epithelial cells. Cytoplasmic dot blot analysis demonstrated that ciliated bronchial epithelial cells had mRNA HLA-DR transcripts, and Northern blot hybridizations showed that the size of the HLA-DR messages was the same observed in other HLA-DR-positive cells. Interestingly, ciliated bronchial epithelial cells showed a significant decline of HLA-DR expression after 5 days in culture, but the addition of gamma-interferon to the cell cultures was associated with the persistence of the expression of class II antigens on the cell surface (P less than 0.01 with control cultures at 5 days). Finally, while ciliated bronchial epithelial cells were ineffective in stimulating allogeneic T cell proliferation in a 6-day primary mixed leukocyte reaction (MLR), the addition of phorbol myristate acetate to the MLR was able to induce a significant T cell proliferation (P less than 0.001, all comparisons). Thus, human ciliated bronchial epithelial cells express HLA-DR surface antigens and have mRNA molecules for the HLA-DR genes, and the expression of the surface class II antigens can be modulated in vitro by immune mediators.(ABSTRACT TRUNCATED AT 400 WORDS)
II类HLA - DR分子由多种非淋巴细胞表达,包括呼吸道上皮细胞。然而,目前尚不清楚纤毛支气管上皮细胞是否表达HLA - DR基因,其表面II类分子的表达是否可被免疫介质调节,以及最终这些细胞是否像其他HLA - DR阳性上皮细胞一样有作为抗原呈递细胞的潜力。为回答这些问题,我们在纤维支气管镜检查期间通过刷取和吸引以及通过刮取手术切除的支气管来收集纤毛支气管上皮细胞。纤维支气管镜检查期间通过刷取或吸引回收的细胞数量相似(P大于0.2),但低于通过刮取手术切除的支气管获得的细胞数量(P小于0.01);然而,与刷取相比,吸引纤毛支气管上皮细胞可获得更好的活力(P小于0.05)。使用PTF 29.12和L243单克隆抗体通过免疫荧光检测纤毛支气管上皮细胞上的HLA - DR抗原,这两种抗体均可识别绝大多数纤毛支气管上皮细胞上的HLA - DR分子。细胞质斑点印迹分析表明纤毛支气管上皮细胞有HLA - DR mRNA转录本,Northern印迹杂交显示HLA - DR信息的大小与在其他HLA - DR阳性细胞中观察到的相同。有趣的是,纤毛支气管上皮细胞在培养5天后HLA - DR表达显著下降,但在细胞培养物中添加γ干扰素与细胞表面II类抗原表达的持续存在相关(与5天的对照培养物相比,P小于0.01)。最后,虽然纤毛支气管上皮细胞在6天的初次混合淋巴细胞反应(MLR)中刺激同种异体T细胞增殖无效,但在MLR中添加佛波醇肉豆蔻酸酯能够诱导显著的T细胞增殖(所有比较,P小于0.001)。因此,人纤毛支气管上皮细胞表达HLA - DR表面抗原并具有HLA - DR基因的mRNA分子,并且表面II类抗原的表达可在体外被免疫介质调节。(摘要截短至400字)
