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大鼠肝脏线粒体载体与谷胱甘肽还原型的窦状隙和胆小管转运体不同的证据。非洲爪蟾卵母细胞中的表达研究。

Evidence that the rat hepatic mitochondrial carrier is distinct from the sinusoidal and canalicular transporters for reduced glutathione. Expression studies in Xenopus laevis oocytes.

作者信息

García-Ruiz C, Morales A, Colell A, Rodés J, Yi J R, Kaplowitz N, Fernández-Checa J C

机构信息

Department of Medicine, Hospital Clinic i Provincial, Universidad de Barcelona, Spain.

出版信息

J Biol Chem. 1995 Jul 7;270(27):15946-9. doi: 10.1074/jbc.270.27.15946.

DOI:10.1074/jbc.270.27.15946
PMID:7608148
Abstract

Mitochondrial GSH derives from a mitochondrial transport system (RmGshT), which translocates cytosol GSH into the mitochondrial matrix. Mitochondria of oocytes, isolated 3-4 days after microinjection of total liver mRNA, expressed a RmGshT compared with water-injected oocytes. The expressed RmGshT exhibited similar functional features as reported in isolated mitochondria of rat liver such as ATP stimulation, inhibition by glutamate, and insensitivity to inhibition by sulfobromophthalein-glutathione (BSP-GSH) and S-(2,4-dinitrophenyl)glutathione (DNP-GSH). The expressed RmGshT is localized in the inner mitochondrial membrane since expression is still observed in mitoplasts prepared from total liver mRNA-injected oocytes. Fractionation of poly(A)+ RNA identified a single mRNA species of approximately 3-3.5 kilobases encoding for the RmGshT, which was stimulated by ATP and inhibited by glutamate but not by BSP-GSH or DNP-GSH. Microinjection of this fraction did not lead to expression of plasma membrane GSH transport in intact oocytes, and conversely, oocytes microinjected with cRNA for rat liver sinusoidal GSH transporter (RsGshT) or rat liver canalicular GSH transporter (RcGshT) did not express mitochondrial GSH transport activity. Thus, our results show the successful expression of the rat hepatic mitochondrial GSH carrier, which is different from RsGshT and RcGshT, and provide the strategic basis for the cloning of this important carrier.

摘要

线粒体谷胱甘肽(GSH)来源于线粒体转运系统(RmGshT),该系统将胞质GSH转运至线粒体基质。在显微注射全肝mRNA 3 - 4天后分离的卵母细胞线粒体,与注射水的卵母细胞相比,表达了一种RmGshT。所表达的RmGshT表现出与大鼠肝脏分离线粒体中报道的类似功能特征,如ATP刺激、谷氨酸抑制,以及对磺溴酞钠 - 谷胱甘肽(BSP - GSH)和S -(2,4 - 二硝基苯基)谷胱甘肽(DNP - GSH)抑制不敏感。所表达的RmGshT定位于线粒体内膜,因为在从注射全肝mRNA的卵母细胞制备的线粒体膜间颗粒中仍可观察到其表达。对聚腺苷酸加尾(poly(A)+)RNA进行分级分离,鉴定出一种约3 - 3.5千碱基的单一mRNA,编码RmGshT,其受ATP刺激,被谷氨酸抑制,但不受BSP - GSH或DNP - GSH抑制。显微注射该组分不会导致完整卵母细胞中质膜GSH转运的表达,相反,用大鼠肝脏窦状GSH转运体(RsGshT)或大鼠肝脏胆小管GSH转运体(RcGshT)的cRNA显微注射的卵母细胞不表达线粒体GSH转运活性。因此,我们的结果表明大鼠肝脏线粒体GSH载体成功表达,它不同于RsGshT和RcGshT,并为克隆这一重要载体提供了策略依据。

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