Mast cells are immune effectors that are localized in tissues, proximal to sites of entry for allergens and other external stimuli. The mediators produced by mast cells are involved in innate immunity against bacteria and parasites, and are key effectors of allergic and asthmatic responses. Mast cell mediators also contribute to fibrosis in asthma, pulmonary fibrosis, scleroderma, and rheumatoid arthritis. The aim of this study was to test the hypothesis that mast cell interactions with fibroblasts are affected by their activation state, in a way that could contribute to the progression of fibrosis. Bone marrow mast cells (BMMC) were derived in vitro from bone marrow progenitors and connective tissue mast cells (CTMC) were harvested from mouse peritoneal cavity. An ELISA was used to measure histamine in the supernatants and cell lysates of activated BMMC and CTMC. Following activation by crosslinking the high affinity IgE receptor, histamine was released from BMMC and CTMC. Starting 24 hours after activation, the total cellular histamine concentration of BMMC was 755+/-14 ng/106 cells, and exceeded the amount in resting BMMC (214+/-9 ng/106 cells). The over-accumulation of histamine peaked 72 hours after activation (3136+/-394 ng/106 cells), and was transient, returning toward the amount in resting BMMC by 96 hours (1787+/-280 ng/106 cells). The increase in histamine was accompanied by an increase in the expression of histidine decarboxylase mRNA, and a 70 kD form of the protein encoded by this mRNA. Similar changes in histamine concentration did not occur in CTMC, indicating that histamine over-accumulation is associated with mast cell phenotype.; To study changes in mast cell adhesion to fibroblasts following activation, an assay was developed to quantify adhesion between mast cells and the NIH-3T3 fibroblast cell line. Resting or activated BMMC or CTMC were cocultured with the fibroblasts for various times to allow adhesion to occur. Nonadherent cells were washed away and adherent mast cells were quantified based on recovery of histamine from the adherent cells. Following activation, adhesion of both BMMC and CTMC to fibroblasts was increased three to six fold. This increased adhesion was not due to increased integrin expression, cell proliferation, or inflammatory mediators released from the mast cells. These findings offer new insights into the role of activated mast cells in fibrotic diseases.
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机译:肥大细胞是免疫效应物,其位于组织中,靠近变应原和其他外部刺激的进入位点。肥大细胞产生的介体参与对细菌和寄生虫的先天免疫,并且是过敏和哮喘反应的关键效应物。肥大细胞介质还导致哮喘,肺纤维化,硬皮病和类风湿性关节炎的纤维化。这项研究的目的是检验肥大细胞与成纤维细胞相互作用受其激活状态影响的假说,其方式可能有助于纤维化的发展。骨髓肥大细胞(BMMC)来源于骨髓祖细胞,结缔组织肥大细胞(CTMC)则来自小鼠腹膜腔。 ELISA用于测量活化的BMMC和CTMC的上清液和细胞裂解物中的组胺。通过交联高亲和力IgE受体激活后,组胺从BMMC和CTMC中释放出来。激活后24小时开始,BMMC的总细胞组胺浓度为755 +/- 14 ng / 106细胞,超过了静息BMMC的浓度(214 +/- 9 ng / 106细胞)。组胺的过度积累在激活后72小时达到峰值(3136 +/- 394 ng / 106个细胞),并且是短暂的,到静止BMMC时达到96个小时(1787 +/- 280 ng / 106个细胞)。组胺的增加伴随着组氨酸脱羧酶mRNA表达的增加,以及由该mRNA编码的70kD形式的蛋白质。在CTMC中未发生类似的组胺浓度变化,表明组胺的过度积累与肥大细胞表型有关。为了研究激活后肥大细胞对成纤维细胞粘附的变化,开发了一种测定法来定量肥大细胞与NIH-3T3成纤维细胞系之间的粘附。将静息或活化的BMMC或CTMC与成纤维细胞共培养不同时间,以使发生粘附。洗去非贴壁细胞,并基于从贴壁细胞中回收的组胺对贴壁肥大细胞进行定量。激活后,BMMC和CTMC对成纤维细胞的粘附力增加了三到六倍。这种增加的粘附不是由于整合素表达增加,细胞增殖或肥大细胞释放的炎性介质而引起的。这些发现为活化的肥大细胞在纤维化疾病中的作用提供了新的见解。
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