Taipei Medical University Institutional Repository:Item 987654321/4915
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    Please use this identifier to cite or link to this item: http://libir.tmu.edu.tw/handle/987654321/4915


    Title: Rosiglitazone在大鼠神經膠質瘤細胞中誘導 Mitogen-Activated Protein Kinase Phosphatase-1 表現的作用機制探討
    The mechanism of rosiglitazone-induced mitogen-activated protein kinase phosphatase-1 expression in rat C6 glioma cells
    Authors: 廖婉茹
    Wan-Ju Liao
    Contributors: 醫學檢驗暨生物技術學研究所
    Keywords: 大鼠神經膠質瘤細胞
    Rosiglitazone
    Mitogen-Activated Protein Kinase Phosphatase-1
    Date: 2005
    Issue Date: 2009-09-10 17:20:35 (UTC+8)
    Abstract: Rosiglitazone(RSG)是一種化學合成的PPAR-γ (peroxisome proliferators-activated receptor-agonist,可用於第二型糖尿病的治療, 它與PPAR-γ具有很強的親和力,為TZDs (thiazolidinediones)類的藥物。RSG還有許多其他的作用,例如: 抗發炎,但其調控的機制目前還不是很清楚。在過去的研究中指出,MKP-1(Mitogen- Activated Protein Kinase Phosphatase-1)能夠使MAPK(Mitogen- Activated Protein Kinase)去活化。為了探討MKP-1在RSG抗發炎反應中扮演的角色,利用RSG處理大鼠神經膠質瘤細胞(C6 glioma),發現RSG會誘導MKP-1表現,在兩小時達到最大量,八小時就回復到原背景值。而以MG-132(蛋白分解?抑制劑)處理,能夠使MKP-1蛋白表現延長至八小時。為了探討RSG調控MKP-1是經由轉錄或轉譯作用,以actinomycin D及cyclohexamide處理皆能抑制由RSG引起的MKP-1表現,表示MKP-1是經由de novo合成而來。為了探討其中的訊息傳遞路徑,利用各種藥理性的抑制劑去抑制ROS、PI3-K、ERK 、NFB,、p38 MAPK、JNK 路徑,發現ERK 1/2抑制劑 (PD098059),NF-B 抑制劑(PDTC)、 p38 MAPK 抑制劑(SB203580) 和JNK抑制劑(SP600125)能夠抑制MKP-1表現,但PI3-K 抑制劑(LY294002)和ROS 抑制劑(l-NAC)不能抑制由 RSG誘導的MKP-1表現,而RSG作用後,磷酸化ERK也明顯上升,表示RSG經由ERK的訊息傳遞路徑而活化MKP-1。在其他研究報告發現,LPS(Lipopolysacchride)可以引起發炎反應,而iNOS可以作為其指標,本篇研究發現RSG可以抑制由LPS所誘導的iNOS表現,而以triptolide (MKP-1 inhibitor) 前處理之後,原先抑制的情況即回復,推斷MKP-1在抗發炎的反應中扮演一個很重要的角色。此外,基質金屬蛋白?(Metalloproteinase ,MMPs)為惡性腫瘤細胞的轉移的一個要素,本研究發現RSG能夠抑制C6 glioma cell 所產生的MMP-2。綜觀以上結果可知MKP-1為細胞內訊息傳遞的調控樞紐,而RSG能夠活化MKP-1而抑制iNOS及MMP-2的表現。
    Rosiglitazone(RSG) or thiazolidinediones is a ligand of the peroxisome proliferators-activated receptor-PPAR-which has been used in the treatment of type II diabetes. Additionally, RSG has been shown to exert a variety of beneficial effects, such as anti-inflammatory. However, the underneath mechanisms are not clear. MAPK phosphatase-1 (MKP-1) has been shown to dephosphorylate and inactivate MAP kinase. To investigate whether MKP-1 plays a role in mediating RSG-induced anti-inflammatory effects. Treatment of C6 glioma cells with RSG, induced a dose-dependent induction of MKP-1, the maximum effect was seen at 2 hours and decreased at 8 hours. Pretreatment with MG-132 prolonged the increasing of MKP-1 protein levels to 8 hours, suggesting RSG may increase MKP-1 stability. To investigate whether RSG regulate the transcription and translation levels of MKP-1, we find that Act. D (actinomycin D) and CHX (cyclohexamide) can inhibit RSG-stimulated MKP-1 expression demonstrated that MKP-1 goes through de novo synthesis. In order to investigate the signaling mechanism, several pharmacological inhibitors were used to block ROS, PI3-K, ERK1/2, NF-B, p38 MAPK and JNK pathways. Pretreatment cells with ERK inhibitor (PD098059), NF-B inhibitor (PDTC), p38 MAPK inhibitor (SB203580) and JNK inhibitor (SP600125) but not PI3-K inhibitor (LY294002) nor ROS blocker(l-NAC) inhibit RSG-stimulated MKP-1 expression. After RSG treatment, phosphorylated- ERK rise was detected. To examine the anti- inflammation role of MKP-1, we demonstrated that RSG can inhibit LPS-induced iNOS expression. Blocking MKP-1 with triptolide reversed iNOS expression. In addition, tumor invasion is regulated by metalloproteinase (MMPs), in our experiments, RSG inhibits MMP-2 mRNA expression. Blocking MKP-1 with triptolide, MMP-2 mRNA expression was reversed. We conclude that RSG exerts anti-inflammatory and MMP-2 inhibition effects through MKP-1 modulation.
    Data Type: thesis
    Appears in Collections:[ ] Dissertations/Theses

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