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大黄酸对人软骨细胞中白细胞介素-1α诱导反应的调节作用:抗体芯片与特异性酶联免疫吸附测定的比较研究

Modulatory effect of rhein on IL-1alpha-induced responses in human chondrocytes: a comparative study between antibody microarrays and specific ELISAs.

作者信息

Deffaud J, Kirchmeyer M, Domagala F, Ficheux H, Netter P, Bianchi A, Jouzeau J-Y

机构信息

UMR 7561 CNRS-Nancy-Université, Laboratoire de Physiopathologie & Pharmacologie Articulaires (LPPA), Vandoeuvre-lès-Nancy, France.

出版信息

Biorheology. 2008;45(3-4):439-55.

PMID:18836244
Abstract

The present work aimed to take advantage of the screening capacity of protein arrays to search for additional targets of rhein in interleukin (IL)-1-stimulated chondrocytes. Primary cultures of chondrocytes from osteoarthritic (OA) patients were stimulated for 24 and 48 h with 1 ng/ml of IL-1alpha, in the presence or absence of 10(-5) M of rhein. Culture supernatants were analyzed with arrays membranes consisting of 120 antibodies directed against cytokines, chemokines, and angiogenic or growth factors and were controlled for 8 proteins by specific immuno-enzymatic assays (ELISA). Protein arrays showed that several CC or CXC chemokines, the growth factor GM-CSF, the cytokines IL-6, IL-7 and IL-10 (but unexpectedly not IL-1beta or TNFalpha) and the adhesion molecule ICAM-1 were induced maximally by IL-1alpha. In IL-1-stimulated chondrocytes, rhein reduced slightly the production of MCP-1 and increased those of IL-1Ra, of the cytokine receptors sgp130, IL-6R, sTNFR I and R II, but also of some chemokines or ICAM-1. Specific ELISAs confirmed the effect of rhein on MCP-1, IL-1Ra, sgp130, IL-6R and sTNFR II but was discrepant for GROalpha and were always more sensitive than protein arrays to detect IL-1 effects such as IL-1Ra and TNFalpha release. The present data show that rhein modulated some IL-1-induced responses contributing possibly to its chondroprotective (IL-1Ra, MCP-1) or cytokine modifying (sTNFR II, sgp130) properties, but that protein arrays were poorly sensitive to check for IL-1- and/or rhein-induced changes.

摘要

本研究旨在利用蛋白质芯片的筛选能力,寻找大黄素在白细胞介素(IL)-1刺激的软骨细胞中的其他作用靶点。从骨关节炎(OA)患者中分离出的原代软骨细胞培养物,在存在或不存在10^(-5) M大黄素的情况下,用1 ng/ml的IL-1α刺激24小时和48小时。用由120种针对细胞因子、趋化因子、血管生成因子或生长因子的抗体组成的芯片膜分析培养上清液,并通过特异性免疫酶测定法(ELISA)对8种蛋白质进行检测。蛋白质芯片显示,几种CC或CXC趋化因子、生长因子GM-CSF、细胞因子IL-6、IL-7和IL-10(但出人意料的是不包括IL-1β或TNFα)以及黏附分子ICAM-1在IL-1α刺激下诱导程度最高。在IL-1刺激的软骨细胞中,大黄素略微降低了MCP-1的产生,并增加了IL-1Ra、细胞因子受体sgp130、IL-6R、sTNFR I和R II的产生,以及一些趋化因子或ICAM-1的产生。特异性ELISA证实了大黄素对MCP-1、IL-1Ra、sgp130、IL-6R和sTNFR II的作用,但对GROα的检测结果不一致,并且在检测IL-1诱导的效应(如IL-1Ra和TNFα释放)方面总是比蛋白质芯片更敏感。目前的数据表明,大黄素调节了一些IL-1诱导的反应,这可能有助于其软骨保护(IL-1Ra、MCP-1)或细胞因子调节(sTNFR II、sgp130)特性,但蛋白质芯片在检测IL-1和/或大黄素诱导的变化方面敏感性较差。

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