LYMPHOCYTE/EPITHELIAL INTERACTIONS IN MUCOSAL REMODELING

粘膜重塑中的淋巴细胞/上皮相互作用

• 批准号: 6781168
• 负责人: CAROL B BASBAUM
• 金额: $ 14.27万
• 依托单位: UNIVERSITY OF CALIFORNIA, SAN FRANCISCO
• 依托单位国家: 美国
• 财政年份: 2003
• 资助国家: 美国
• 起止时间: 2003-07-01 至 2004-06-30
• 项目状态: 已结题
• 来源: https://reporter.nih.gov/project-details/6781168
• 关键词: JAK kinase; Mycoplasma; asthma; biomarker; bronchial mucus; cell cell interaction; cell differentiation; cell population study; cellular pathology; collagenase; flow cytometry; gel mobility shift assay; immunocytochemistry; immunofluorescence technique; inflammation; interleukin 9; laboratory mouse; lymphocyte; metalloendopeptidases; mucins; mycoplasmal pneumonia; polymerase chain reaction; respiratory epithelium; respiratory infections; transcription factor

The epithelium of chronically inflamed airways is characterized by mucus hypersecretion and shows 2 relevant adaptations: (a) mucous cell metaplasia, whereby individual epithelial cells differentiate to express mucin and (b) epithelial remodeling whereby the entire epithelial tissue layer becomes convoluted, invading connective tissue to form mucous crypts and glands. To identify molecular mechanisms underlying these changes requires the use of biochemical markers. Mucin can be considered a marker for mucous metaplasia as mucous differentiation is dependent on mucin gene expression. Metalloproteinases can be considered markers for epithelial remodeling as morphogenetic processes requiring connective tissue degradation are dependent on these enzymes. Seeking stimuli potentially controlling mucin and metalloproteinase expression in the inflamed airway we tested the effect of lymphocyte-derived cytokines. Product of both mixed lymphocyte reactions and fluid from asthmatic airways stimulated expression of the two markers at the RNA level. Experiments described below indicate that the Th2 cell mediator IL-9 is a major mucin stimulus in asthmatic airway fluid and that the T cell surface marker OX-47 (EMMPRIN) strongly stimulates metalloproteinases 1 and 9. Based on these relationships, we hypothesize that activated T cells in inflamed airways control mucous metaplasia and epithelial remodeling via IL-9 and EMMPRIN. Specific aim 1 will use mutant mice to determine which lymphocyte populations are required for M. pulmonis-induced mucin (Muc 5ac) and metalloproteinase (MMP-9) gene activation. Specific aim 2, using chemical inhibitors, dominant negative mutants and chimeric IL-9 receptor constructs, will test the hypothesis that IL-9 stimulates MUC5 AC in human bronchial epithelial cells via intersecting JAK-STAT and MAPK signaling pathways. Specific aim 3, using biochemical inhibitors, dominant negative mutants and a novel mutagenesis approach, will test the hypothesis that EMMPRIN stimulates MMP-1 in human fibroblasts via a p38-dependent mechanisms and will identify key elements of EMMPRIN-MMP signaling.

慢性炎症气道的上皮的特征在于粘液分泌过多，并显示2种相关适应：（a）粘液细胞化生，由此个体上皮细胞分化以表达粘蛋白，和（B）上皮重塑，由此整个上皮组织层变得卷曲，侵入结缔组织以形成粘液隐窝和腺体。 为了确定这些变化背后的分子机制，需要使用生化标记物。 粘蛋白可以被认为是粘液化生的标志物，因为粘液分化依赖于粘蛋白基因表达。金属蛋白酶可以被认为是上皮重塑的标志物，因为需要结缔组织降解的形态发生过程依赖于这些酶。寻找潜在控制炎症气道中粘蛋白和金属蛋白酶表达的刺激，我们测试了淋巴细胞衍生的细胞因子的作用。混合淋巴细胞反应产物和哮喘气道液体刺激了这两种标记物在RNA水平的表达。 下述实验表明，Th 2细胞介体IL-9是哮喘气道液中的主要粘蛋白刺激物，T细胞表面标志物OX-47（EMMPRIN）强烈刺激金属蛋白酶1和9。 基于这些关系，我们假设炎症气道中活化的T细胞通过IL-9和EMMPRIN控制粘膜化生和上皮重塑。具体目标1将使用突变小鼠来确定M所需的淋巴细胞群。肺结核诱导的粘蛋白（Muc 5ac）和金属蛋白酶（MMP-9）基因活化。 具体目标2，使用化学抑制剂、显性失活突变体和嵌合IL-9受体构建体，将测试IL-9通过交叉JAK-STAT和MAPK信号传导途径刺激人支气管上皮细胞中的MUC 5 AC的假设。 具体目标3，使用生化抑制剂，显性负突变体和一种新的诱变方法，将测试EMMPRIN通过p38依赖性机制刺激人成纤维细胞中MMP-1的假设，并将确定EMMPRIN-MMP信号传导的关键要素。