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血红素加氧酶-1基因的表达对由佛波醇(一种谷胱甘肽耗竭剂)在大鼠肝脏中产生的氧化应激作出反应;与c-jun氨基末端激酶激活的相关性。

The expression of heme oxygenase-1 gene responded to oxidative stress produced by phorone, a glutathione depletor, in the rat liver; the relevance to activation of c-jun n-terminal kinase.

作者信息

Oguro T, Hayashi M, Nakajo S, Numazawa S, Yoshida T

机构信息

Department of Biochemical Toxicology, School of Pharmaceutical Sciences, Showa University, 1-5-8 Hatanodai, Shinagawa-ku, Tokyo 142, Japan.

出版信息

J Pharmacol Exp Ther. 1998 Nov;287(2):773-8.

PMID:9808709
Abstract

Phorone, a glutathione (GSH) depletor, induces the expression of mRNAs of heme oxygenase-1 (HO-1) and c-jun by mediating the activation of activated protein-1 (AP-1) in rat livers. We have shown that phorone activates c-Jun N-terminal kinase (JNK), thus leading to c-Jun phosphorylation, and transactivation of AP-1 and HO-1 gene expression in the rat liver in response to oxidative stress. The in-gel kinase assay showed that phorone activated JNK1 predominantly in the rat liver nuclear extract. The JNK activation by phorone was slightly observed at 1 hr after administration and gradually increased with time. Ser73-phosphorylation of c-Jun catalyzed by JNK was significantly altered by changing hepatic GSH levels based on the results observed by the combined injection of buthionine sulfoximine (BSO) or GSH isopropyl ester (GIP) with phorone. Namely, BSO, an inhibitor of GSH biosynthesis, enhanced phorone-mediated c-Jun phosphorylation as well as AP-1 binding activity. However, GSH isopropyl ester prevented GSH depletion and abolished both c-Jun phosphorylation and the activation of AP-1 binding evoked by phorone. GSH isopropyl ester also suppressed phorone-produced HO-1 and c-jun gene expressions to 25 and 30% of the induced level. Perfluorodecanoic acid (PFDA) reduced GSH S-transferase activity, prevented phorone-mediated GSH depletion and abolished either HO-1 or c-jun mRNA induction by phorone. These results indicated that oxidative stress under GSH depletion produced by phorone could activate preferentially JNK and lead to the transcriptional activation of AP-1 and consequently to HO-1 gene expression. This study suggests that JNK activation could be one of the major signaling pathways to transmit intracellular events to the nuclei during oxidative stress via GSH depletion by phorone in rat livers.

摘要

二甲基庚二酮,一种谷胱甘肽(GSH)耗竭剂,通过介导大鼠肝脏中活化蛋白-1(AP-1)的激活来诱导血红素加氧酶-1(HO-1)和c-jun的mRNA表达。我们已经表明,二甲基庚二酮激活c-Jun氨基末端激酶(JNK),从而导致c-Jun磷酸化,并在大鼠肝脏中响应氧化应激而激活AP-1和HO-1基因表达。凝胶内激酶分析表明,二甲基庚二酮主要在大鼠肝脏核提取物中激活JNK1。给药后1小时可轻微观察到二甲基庚二酮对JNK的激活作用,且随时间逐渐增加。根据丁硫氨酸亚砜胺(BSO)或谷胱甘肽异丙酯(GIP)与二甲基庚二酮联合注射的观察结果,改变肝脏GSH水平会显著改变JNK催化的c-Jun的Ser73磷酸化。也就是说,BSO,一种GSH生物合成抑制剂,增强了二甲基庚二酮介导的c-Jun磷酸化以及AP-1结合活性。然而,谷胱甘肽异丙酯可防止GSH耗竭,并消除二甲基庚二酮引起的c-Jun磷酸化和AP-1结合激活。谷胱甘肽异丙酯还将二甲基庚二酮产生的HO-1和c-jun基因表达抑制到诱导水平的25%和30%。全氟癸酸(PFDA)降低了GSH S-转移酶活性,防止了二甲基庚二酮介导的GSH耗竭,并消除了二甲基庚二酮对HO-1或c-jun mRNA的诱导。这些结果表明,二甲基庚二酮产生的GSH耗竭下的氧化应激可优先激活JNK,并导致AP-1的转录激活,进而导致HO-1基因表达。本研究表明,JNK激活可能是氧化应激期间通过二甲基庚二酮使大鼠肝脏GSH耗竭将细胞内事件传递至细胞核的主要信号通路之一。

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