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慢性黏膜炎症性疾病中上皮抗原致敏。体外对与纯化上皮细胞相关成分反应的人肠黏膜来源单核细胞的特性研究。

Sensitization to epithelial antigens in chronic mucosal inflammatory disease. Characterization of human intestinal mucosa-derived mononuclear cells reactive with purified epithelial cell-associated components in vitro.

作者信息

Roche J K, Fiocchi C, Youngman K

出版信息

J Clin Invest. 1985 Feb;75(2):522-30. doi: 10.1172/JCI111728.

DOI:10.1172/JCI111728
PMID:3871793
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC423527/
Abstract

To explore the auto-reactive potential of cells infiltrating the gut mucosa in idiopathic chronic inflammatory bowel disease, intestinal lamina propria mononuclear cells (LPMC) were isolated, characterized morphologically and phenotypically, and evaluated for antigen-specific reactivity. The last was assessed by quantitating LPMC cytotoxic capabilities against purified, aqueous-soluble, organ-specific epithelial cell-associated components (ECAC) characterized previously. Enzyme-isolated inflammatory bowel disease LPMC were constituted primarily by T lymphocytes (57 +/- 12% OKT 3-positive), B lymphocytes (18 +/- 9% surface immunoglobulin-positive), and macrophages (11 +/- 6% esterase-positive), and were responsive to phytohemagglutinin (mean uptake 86,933 cpm/5 X 10(5) cells). LPMC present in abnormal segments from 71% of patients with chronic inflammatory bowel disease were cytotoxic for ECAC isolated from colon (12.5 +/- 8.9% specific lysis) and small bowel (7.1 +/- 6.5%), but not for kidney control antigen (0.8 +/- 1.1%) isolated in a manner analogous to that used for ECAC (P less than 0.02). In contrast, despite comparable responses to phytohemagglutinin (mean uptake 59,200 cpm/5 X 10(5) cells), LPMC from histologically normal mucosa of patients with benign (adult megacolon, Hirshsprung's disease, diverticulosis) or malignant disease failed to lyse indicator cells labeled with colon-derived ECAC (0.3 +/- 0.08%), small bowel-derived ECAC (0.4 +/- 1.11%), or kidney antigen (0.29 +/- 0.79%). LPMC reactivity for individual gel-purified macromolecules of small bowel-derived ECAC (designated as the "P" series of components) was greatest against component P1 (by 2-3-fold), but was detectable against three other purified components as well. The addition of patient's serum did not enhance cytotoxicity to ECAC. Characterization of the cytotoxic cell showed that it was nonadherent to plastic surfaces, bore T lymphocyte-specific markers detectable by OKT 11 and OKT 3 monoclonal antibodies, and could be depleted by removal of cells with receptors for sheep erythrocytes. ECAC-specific reactivity was markedly reduced (greater than 93%) in most experiments when LPMC were preincubated for 1 h with ECAC. These data support the concept that autosensitization to several epithelial cell-associated components has occurred in patients with chronic inflammatory bowel disease, and provide initial evidence that antigen-specific, cell-mediated mechanisms may play a role in the pathogenesis of these disorders.

摘要

为探究特发性慢性炎症性肠病中浸润肠道黏膜的细胞的自身反应潜能,分离了肠固有层单核细胞(LPMC),对其进行形态学和表型特征分析,并评估其抗原特异性反应性。通过定量LPMC对先前鉴定的纯化、水溶性、器官特异性上皮细胞相关成分(ECAC)的细胞毒性能力来评估后者。酶分离的炎症性肠病LPMC主要由T淋巴细胞(57±12% OKT 3阳性)、B淋巴细胞(18±9%表面免疫球蛋白阳性)和巨噬细胞(11±6%酯酶阳性)组成,并对植物血凝素产生反应(平均摄取量86,933 cpm/5×10⁵个细胞)。71%的慢性炎症性肠病患者异常节段中的LPMC对从结肠分离的ECAC(特异性裂解率12.5±8.9%)和小肠分离的ECAC(7.1±6.5%)具有细胞毒性,但对以与ECAC类似方式分离的肾脏对照抗原(0.8±1.1%)无细胞毒性(P<0.02)。相比之下,尽管对植物血凝素的反应相当(平均摄取量59,200 cpm/5×10⁵个细胞),但来自良性(成人巨结肠、先天性巨结肠、憩室病)或恶性疾病患者组织学正常黏膜的LPMC未能裂解用结肠来源的ECAC(0.3±0.08%)、小肠来源的ECAC(0.4±1.11%)或肾脏抗原(0.29±0.79%)标记的指示细胞。LPMC对小肠来源的ECAC的单个凝胶纯化大分子(指定为“P”系列成分)的反应性对成分P1最大(高2 - 3倍),但对其他三种纯化成分也可检测到反应。添加患者血清并未增强对ECAC的细胞毒性。细胞毒性细胞的特征表明,它不黏附于塑料表面,带有可被OKT 11和OKT 3单克隆抗体检测到的T淋巴细胞特异性标志物,并且通过去除具有绵羊红细胞受体的细胞可使其减少。在大多数实验中,当LPMC与ECAC预孵育1小时时,ECAC特异性反应性显著降低(>93%)。这些数据支持了慢性炎症性肠病患者已对几种上皮细胞相关成分发生自身致敏的概念,并提供了初步证据表明抗原特异性细胞介导机制可能在这些疾病的发病机制中起作用。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7cf8/423527/5d7c988ea404/jcinvest00119-0218-a.jpg
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https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7cf8/423527/5d7c988ea404/jcinvest00119-0218-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7cf8/423527/367dde46c54c/jcinvest00119-0217-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7cf8/423527/5d7c988ea404/jcinvest00119-0218-a.jpg

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