Department of Rheumatology, St. Vincent's University Hospital, Dublin Academic Healthcare, Dublin, Ireland.
PLoS One. 2011;6(8):e24048. doi: 10.1371/journal.pone.0024048. Epub 2011 Aug 24.
This study examines the expression of IL-17A-secreting cells within the inflamed synovium and the relationship to in vivo joint hypoxia measurements.
IL-17A expression was quantified in synovial tissue (ST), serum and synovial fluid (SF) by immunohistochemistry and MSD-plex assays. IL-6 SF and serum levels were measured by MSD-plex assays. Dual immunofluorescence for IL-17A was quantified in ST CD15+ cells (neutrophils), Tryptase+ (mast cells) and CD4+ (T cells). Synovial tissue oxygen (tpO(2)) levels were measured under direct visualisation at arthroscopy. Synovial infiltration was assessed using immunohistochemistry for cell specific markers. Peripheral blood mononuclear and polymorphonuclear cells were isolated and exposed to normoxic or 3% hypoxic conditions. IL-17A and IL-6 were quantified as above in culture supernatants.
IL-17A expression was localised to mononuclear and polymorphonuclear (PMN) cells in inflamed ST. Dual immunoflourescent staining co-localised IL-17A expression with CD15+ neutrophils Tryptase+ mast cells and CD4+T cells. % IL-17A positivity was highest on CD15+ neutrophils, followed by mast cells and then CD4+T-cells. The number of IL-17A-secreting PMN cells significantly correlated with sublining CD68 expression (r = 0.618, p<0.01). IL-17A SF levels correlated with IL-6 SF levels (r = 0.675, p<0.01). Patients categorized according to tp0(2)< or >20 mmHg, showed those with low tp0(2)<20 mmHg had significantly higher IL-17A+ mononuclear cells with no difference observed for PMNs. Exposure of mononuclear and polymorphonuclear cells to 3% hypoxia, significantly induced IL-6 in mononuclear cells, but had no effect on IL-17A expression in mononuclear and polymorphonuclear cells.
This study demonstrates IL-17A expression is localised to several immune cell subtypes within the inflamed synovial tissue, further supporting the concept that IL-17A is a key mediator in inflammatory arthritis. The association of hypoxia with Il-17A expression appears to be indirect, probably through hypoxia-induced pro-inflammatory pathways and leukocyte influx within the joint microenvironment.
本研究探讨了 IL-17A 分泌细胞在炎症滑膜中的表达及其与体内关节缺氧测量的关系。
通过免疫组织化学和 MSD 多指标检测法,对滑膜组织(ST)、血清和滑液(SF)中的 IL-17A 表达进行定量分析。通过 MSD 多指标检测法测量 SF 和血清中 IL-6 水平。通过 IL-17A 的双重免疫荧光,对 ST 中 CD15+细胞(中性粒细胞)、Tryptase+(肥大细胞)和 CD4+(T 细胞)中的 IL-17A 进行定量分析。在关节镜直视下测量滑膜组织的氧(tpO(2))水平。使用针对细胞特异性标志物的免疫组织化学评估滑膜浸润情况。分离外周血单核细胞和多形核细胞,并将其暴露于正常氧或 3%缺氧条件下。通过上述方法检测培养上清液中的 IL-17A 和 IL-6。
IL-17A 表达定位于炎症 ST 的单核细胞和多形核细胞(PMN)中。双重免疫荧光染色显示 IL-17A 表达与 CD15+中性粒细胞、Tryptase+肥大细胞和 CD4+T 细胞共定位。CD15+中性粒细胞上的 IL-17A 阳性率最高,其次是肥大细胞,然后是 CD4+T 细胞。分泌 IL-17A 的 PMN 细胞数量与亚衬里 CD68 表达呈显著正相关(r=0.618,p<0.01)。SF 中 IL-17A 水平与 SF 中 IL-6 水平呈正相关(r=0.675,p<0.01)。根据 tp0(2)<或>20mmHg 对患者进行分类,tp0(2)<20mmHg 的低氧患者中,IL-17A+单核细胞明显增加,但 PMN 中未见差异。将单核细胞和多形核细胞暴露于 3%缺氧环境中,单核细胞中显著诱导了 IL-6 的表达,但对单核细胞和多形核细胞中 IL-17A 的表达没有影响。
本研究表明,IL-17A 表达定位于炎症滑膜组织中的几种免疫细胞亚型,进一步支持 IL-17A 是炎症性关节炎的关键介质这一概念。缺氧与 Il-17A 表达的关联似乎是间接的,可能是通过缺氧诱导的促炎途径和关节微环境中的白细胞浸润。
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