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对不同的核因子κB蛋白进行调控会改变白细胞介素-1β诱导的人类风湿性滑膜成纤维细胞前列腺素E2的生成。

Manipulation of distinct NFkappaB proteins alters interleukin-1beta-induced human rheumatoid synovial fibroblast prostaglandin E2 formation.

作者信息

Roshak A K, Jackson J R, McGough K, Chabot-Fletcher M, Mochan E, Marshall L A

机构信息

SmithKline Beecham Pharmaceuticals, SmithKline Beecham Pharmaceuticals, Immunopharmacology, UW2532, King of Prussia, Pennsylvania 19406, USA.

出版信息

J Biol Chem. 1996 Dec 6;271(49):31496-501. doi: 10.1074/jbc.271.49.31496.

DOI:10.1074/jbc.271.49.31496
PMID:8940164
Abstract

Interleukin 1beta (IL-1beta) up-regulates human rheumatoid synovial fibroblast (RSF) 85-kDa phospholipase A2 (PLA2) and mitogen-inducible cyclooxygenase (COX) II. Promoter regions for these genes contain a motif that closely resembles the "classic" NFkappaB consensus site. Immunoblot analysis identified NFkappaB1 (p50), RelA (p65), and c-Rel in RSF. Upon IL-1beta-stimulation, p65 and c-Rel but not p50 protein levels were reduced suggesting nuclear translocation. IL-1beta-induced RSF nuclear extracts contained a p65-containing complex, which bound to the classical NFkappaB consensus motif. An NFkappaB classical oligonucleotide decoy produced a concentration-dependent decrease in IL-1-stimulated PGE2 production (IC50 = approximately 2 microM), indicating a role of NFkappaB. Utilization of antisense technology showed that p65 but not p50 or c-Rel mediated IL-1beta-stimulated PGE2 formation. Treated RSF could not transcribe COX II or 85-kDa PLA2 mRNA, which reduced their respective proteins. Interestingly, stimulated IL-8 production was not inhibited by the classical NFkappaB decoy but was reduced by treatment with antisense to both p65 and c-Rel supporting preferential binding of c-Rel-p65 to the "alternative" IL-8 kappaB motif. Taken together, these data provide the first direct evidence for a role of p65 in COX II and 85-kDa PLA2 gene induction and support the IL-1 activation and participation of distinct NFkappaB protein dimers in RSF prostanoid and IL-8 formation.

摘要

白细胞介素1β(IL-1β)上调人类风湿性滑膜成纤维细胞(RSF)的85 kDa磷脂酶A2(PLA2)和丝裂原诱导型环氧化酶(COX)II。这些基因的启动子区域含有一个与“经典”NFκB共有序列非常相似的基序。免疫印迹分析在RSF中鉴定出NFκB1(p50)、RelA(p65)和c-Rel。在IL-1β刺激后,p65和c-Rel的蛋白水平降低而p50未降低,提示发生了核转位。IL-1β诱导的RSF核提取物含有一个含p65的复合物,其与经典的NFκB共有基序结合。一种NFκB经典寡核苷酸诱饵导致IL-1刺激的前列腺素E2产生呈浓度依赖性降低(IC50 = 约2 μM),表明NFκB发挥了作用。利用反义技术显示,p能介导IL-1β刺激的前列腺素E2形成,而p50或c-Rel则不能。经处理的RSF无法转录COX II或85 kDa PLA2 mRNA,从而降低了它们各自的蛋白水平。有趣的是,经典的NFκB诱饵并未抑制IL-8的产生,但用针对p65和c-Rel的反义核酸处理可使其降低,这支持了c-Rel-p65与“替代性 ”IL-8 κB基序的优先结合。综上所述,这些数据首次直接证明了p65在COX II和85 kDa PLA2基因诱导中的作用,并支持了IL-1激活以及不同的NFκB蛋白二聚体参与RSF中前列腺素和IL-8形成的过程。 65

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