François Mathias, Richette Pascal, Tsagris Lydia, Fitting Catherine, Lemay Cedric, Benallaoua Mourad, Tahiri Khadija, Corvol Marie-Therese
INSERM UMR-S-530-747, University Paris Descartes, Paris, France.
Arthritis Rheum. 2006 Apr;54(4):1233-45. doi: 10.1002/art.21728.
To determine whether peroxisome proliferator-activated receptor alpha (PPARalpha) agonists protect chondrocytes against the effects of interleukin-1beta (IL-1beta).
PPARalpha expression and function in cultured rabbit articular chondrocytes were studied by Northern blotting, electrophoretic mobility shift assay, and transient expression of a luciferase reporter construct bearing the human IL-1 receptor antagonist (Il-1Ra) gene promoter. Chondrocytes were incubated in vitro with IL-1beta alone or in combination with CloFibrate (CloF) or other PPAR ligands. Proteoglycans were evaluated by 35S-sulfate incorporation, matrix metalloproteinase (MMP) levels were assessed by zymography and enzyme-linked immunosorbent assay (ELISA), and MMP messenger RNA (mRNA) levels were measured by Northern blotting and real-time reverse transcriptase-polymerase chain reaction. IL-1beta and IL-1Ra soluble contents were measured by ELISA.
CloF counteracted IL-1beta-induced 35S-proteoglycan degradation, gelatinolytic activity, and MMP-1, -3, and -13 mRNA expression. CloF also maximized IL-1beta-induced endogenous production of soluble IL-1Ra (sIL-1Ra). This stimulating effect on IL-1Ra gene expression was shown, by transient expression assay, to be transcriptional. Inhibition of sIL-1Ra expression by a specific small interfering RNA suppressed the effect of CloF on IL-1beta-induced MMP expression. The stimulatory effect of CloF was enhanced by cotransfection with wild-type PPARalpha and abolished by a dominant-negative PPARalpha mutant. Fenofibrate and WY-14643 displayed a similar stimulating effect on the IL-1Ra promoter, while rosiglitazone did not. Two PPAR response elements, an NF-kappaB-binding site, and a CCAAT/enhancer binding protein-binding site were identified in the IL-1Ra promoter. All 4 sites were necessary for mediation of the effects of CloF.
Our findings support the notion that there is a PPARalpha-dependent mechanism that inhibits IL-1beta function in chondrocytes, which operates via an increase in sIL-1Ra production.
确定过氧化物酶体增殖物激活受体α(PPARα)激动剂是否能保护软骨细胞免受白细胞介素-1β(IL-1β)的影响。
通过Northern印迹法、电泳迁移率变动分析以及携带人白细胞介素-1受体拮抗剂(Il-1Ra)基因启动子的荧光素酶报告构建体的瞬时表达,研究培养的兔关节软骨细胞中PPARα的表达和功能。软骨细胞在体外单独与IL-1β孵育,或与氯贝丁酯(CloF)或其他PPAR配体联合孵育。通过35S-硫酸盐掺入评估蛋白聚糖,通过酶谱分析和酶联免疫吸附测定(ELISA)评估基质金属蛋白酶(MMP)水平,通过Northern印迹法和实时逆转录聚合酶链反应测量MMP信使核糖核酸(mRNA)水平。通过ELISA测量IL-1β和IL-1Ra的可溶性含量。
CloF抵消了IL-1β诱导的35S-蛋白聚糖降解、明胶酶活性以及MMP-1、-3和-13 mRNA表达。CloF还使IL-1β诱导的可溶性IL-1Ra(sIL-1Ra)内源性产生最大化。通过瞬时表达分析表明,这种对IL-1Ra基因表达的刺激作用是转录性的。用特异性小干扰RNA抑制sIL-1Ra表达可抑制CloF对IL-1β诱导的MMP表达的作用。与野生型PPARα共转染可增强CloF的刺激作用,而显性负性PPARα突变体则可消除该作用。非诺贝特和WY-14643对IL-1Ra启动子显示出类似的刺激作用,而罗格列酮则没有。在IL-1Ra启动子中鉴定出两个PPAR反应元件、一个NF-κB结合位点和一个CCAAT/增强子结合蛋白结合位点。所有这4个位点对于介导CloF的作用都是必需的。
我们的研究结果支持这样一种观点,即存在一种PPARα依赖性机制,该机制通过增加sIL-1Ra的产生来抑制软骨细胞中IL-1β的功能。
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