Center for the Study and Cure of Coeliac Disease, IRCCS Policlinico San Matteo Foundation, University of Pavia, Italy.
Int J Immunopathol Pharmacol. 2010 Jan-Mar;23(1):179-91. doi: 10.1177/039463201002300116.
Tissue transglutaminase (TG2) was identified as the humoral autoantigen in coeliac disease, but whether it can also serve as T cell autoantigen is still unknown. We aimed, therefore, to firstly explore the presence of TG2-specific T cells in peripheral blood of ten adult patients (four active, i.e. carrying both serological and histological features of the disease; four treated, i.e. with proven mucosal recovery and disappearance of specific antibodies after an adequate period of gluten free diet; and two potential coeliacs, i.e. carrying the serological stigmata of the disease, but not the intestinal lesions), and four healthy controls (two carrying the HLA-DQ2 haplotype of susceptibility to the disease), and secondly to carry out a detailed in vitro characterization of the isolated antigen-specific T cells. T cell lines were first established by means of weekly stimulation with human recombinant TG2 followed by generation of T cell clones through distribution of T cells on plates at one cell/well limiting dilution and further rounds of stimulation. Antigen specificity and HLA-DQ2 restriction were both assessed by evaluating the proliferative response to TG2 in the absence and presence of human sera blocking HLA-DQ2 molecules, after exclusion of impurities in the antigen preparation. Immune phenotyping of T cell clones was performed by flow cytometry, and the expression of IL-1â, IL-4, IL-6, IL-10, IL-12, TGF-beta, IFN-gamma and TNF-alpha was determined by ELISA assay on the supernatants of these clones. A total of 91 T cell clones were isolated from the three HLA-DQ2-positive, active patients, but none from the other patients and controls. The immune phenotyping showed that the majority of them (85.7 percent) were CD3/CD4+ and only a small percentage (14.3 percent) were CD3/CD8+, all carried the TCR alphabeta, and had a memory phenotype. The cytokine profile showed high levels of IFN-gamma and IL-6 that, together with the absence of IL-4, placed these T cell clones in the T helper type 1-like category. Further in vitro analysis was carried out on 32/91 CD4+ clones and showed a specific and dose-dependent proliferative response towards TG2 and an HLA-DQ2 restriction. Finally, when incubating duodenal mucosal specimens of treated patients with the supernatant of TG2-specific T cell clones, characteristic disease lesions were found, indicating a role for TG2-specific cellular immune response in the pathogenesis of coeliac disease.
组织转谷氨酰胺酶(TG2)已被确定为乳糜泻中的体液自身抗原,但它是否也可以作为 T 细胞自身抗原尚不清楚。因此,我们旨在首先探索十名成年患者(四名活动期,即既具有血清学和组织学特征,又具有疾病;四名治疗期,即经过充分的无麸质饮食治疗后黏膜恢复,特异性抗体消失;两名潜在的乳糜泻患者,即具有疾病的血清学标志,但没有肠道病变)和四名健康对照者(两名携带易患疾病的 HLA-DQ2 单倍型)外周血中是否存在 TG2 特异性 T 细胞;其次,对分离的抗原特异性 T 细胞进行详细的体外特征描述。通过每周用重组人 TG2 刺激,然后在平板上分配 T 细胞进行克隆,将 T 细胞克隆化,以建立 T 细胞系,在没有和存在阻断 HLA-DQ2 分子的人血清的情况下,评估对 TG2 的增殖反应,以排除抗原制备中的杂质。通过流式细胞术对 T 细胞克隆进行免疫表型分析,并通过 ELISA 测定这些克隆上清液中 IL-1â、IL-4、IL-6、IL-10、IL-12、TGF-β、IFN-γ和 TNF-α的表达。从三名 HLA-DQ2 阳性、活动期患者中分离出 91 个 T 细胞克隆,但其他患者和对照组中均未分离出。免疫表型分析表明,它们中的大多数(85.7%)为 CD3/CD4+,只有一小部分(14.3%)为 CD3/CD8+,均携带 TCR alphabeta,具有记忆表型。细胞因子谱显示高水平的 IFN-γ和 IL-6,加上缺乏 IL-4,将这些 T 细胞克隆归类为辅助性 T 细胞 1 样。对 91 个 CD4+克隆中的 32 个进行进一步的体外分析,结果显示对 TG2 具有特异性和剂量依赖性的增殖反应,以及 HLA-DQ2 限制。最后,当用 TG2 特异性 T 细胞克隆的上清液孵育治疗患者的十二指肠黏膜标本时,发现特征性病变,表明 TG2 特异性细胞免疫反应在乳糜泻发病机制中起作用。
