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评估前列腺素E2对重组马白细胞介素-1β刺激的马软骨细胞培养物中基质金属蛋白酶1、3和13以及基质金属蛋白酶组织抑制剂1表达的影响。

Evaluation of the influence of prostaglandin E2 on recombinant equine interleukin-1beta-stimulated matrix metalloproteinases 1, 3, and 13 and tissue inhibitor of matrix metalloproteinase 1 expression in equine chondrocyte cultures.

作者信息

Tung Jayne T, Arnold Carolyn E, Alexander Lee H, Yuzbasiyan-Gurkan Vilma, Venta Patrick J, Richardson Dean W, Caron John P

机构信息

Department of Large Animal Clinical Sciences, Michigan State University, East Lansing 48824, USA.

出版信息

Am J Vet Res. 2002 Jul;63(7):987-93. doi: 10.2460/ajvr.2002.63.987.

DOI:10.2460/ajvr.2002.63.987
PMID:12118680
Abstract

OBJECTIVE

To determine the effects of prostaglandin E2 (PGE2) on recombinant equine interleukin (IL)-1beta-stimulated expression of matrix metalloproteinases (MMP 1, MMP 3, MMP 13) and tissue inhibitor of matrix metalloproteinase 1 (TIMP 1) in vitro.

SAMPLE POPULATION

Cultured equine chondrocytes.

PROCEDURE

Stationary monolayers of first-passage chondrocytes were exposed to graduated concentrations of PGE2 with or without a subsaturating dose (50 pg/ml) of recombinant equine IL-1beta (reIL-1beta) to induce expression of MMP 1, MMP 3, MMP 13, and TIMP 1, followed by RNA isolation and northern blotting. In subsequent experiments, gene expression was similarly quantified from mRNA isolated from cultures pretreated with phenylbutazone to quench endogenous PGE2 synthesis, followed by exposure to reIL-1beta and exogenous PGE2 (5 mg/ml) with appropriate controls.

RESULTS

Exogenous PGE2 (10 mg/ml) significantly reduced reIL-1beta-induced expression of MMP 1, MMP 3, MMP 13, and TIMP 1. Abrogation of cytokine induction with this dose of PGE2 was comparable to that for dexamethasone (10(-5) M) control. Similarly, pretreatment with phenylbutazone, followed by exposure to relL-1beta and PGE2 (5 mg/ml), was associated with a reduced expression of the genes of interest, an effect that was significant for MMP 1, MMP 13, and TIMP 1.

CONCLUSIONS AND CLINICAL RELEVANCE

The MMP and TIMP 1 are important mediators in the pathophysiologic events in osteoarthritis. The potential for physiologically relevant regulation of expression of these genes by PGE2 is a consideration in the use of drugs that inhibit prostanoid synthesis in the treatment of equine arthropathies.

摘要

目的

在体外确定前列腺素E2(PGE2)对重组马白细胞介素(IL)-1β刺激的基质金属蛋白酶(MMP 1、MMP 3、MMP 13)和基质金属蛋白酶组织抑制剂1(TIMP 1)表达的影响。

样本群体

培养的马软骨细胞。

实验步骤

将第一代软骨细胞的静止单层细胞暴露于不同浓度的PGE2,有或没有亚饱和剂量(50 pg/ml)的重组马IL-1β(reIL-1β),以诱导MMP 1、MMP 3、MMP 13和TIMP 1的表达,随后进行RNA分离和Northern印迹分析。在随后的实验中,同样从用保泰松预处理以抑制内源性PGE2合成的培养物中分离出的mRNA中定量基因表达,然后暴露于reIL-1β和外源性PGE2(5 mg/ml)并设置适当对照。

结果

外源性PGE2(10 mg/ml)显著降低reIL-1β诱导的MMP 1、MMP 3、MMP 13和TIMP 1的表达。该剂量的PGE2对细胞因子诱导的消除作用与地塞米松(10⁻⁵ M)对照相当。同样,用保泰松预处理,然后暴露于relL-1β和PGE2(5 mg/ml),与目标基因表达降低有关,这一作用对MMP 1、MMP 13和TIMP 1具有显著意义。

结论及临床意义

MMP和TIMP 1是骨关节炎病理生理事件中的重要介质。在使用抑制前列腺素合成的药物治疗马关节病时,需考虑PGE2对这些基因表达进行生理相关调节的可能性。

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