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首页> 外文期刊>Archives of Biochemistry and Biophysics >Enrichment and functional reconstitution of glutathione transport activity from rabbit kidney mitochondria: Further evidence for the role of the dicarboxylate and 2-oxoglutarate carriers in mitochondrial glutathione transport
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Enrichment and functional reconstitution of glutathione transport activity from rabbit kidney mitochondria: Further evidence for the role of the dicarboxylate and 2-oxoglutarate carriers in mitochondrial glutathione transport

机译:兔肾脏线粒体中谷胱甘肽转运活性的富集和功能重建:二羧酸盐和2-氧戊二酸载体在线粒体谷胱甘肽转运中的作用的进一步证据

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In previous studies, we provided evidence for uptake of glutathione (GSH) by the dicarboxylate and the a-oxoglutarate carriers in rat kidney mitochondria, To investigate further the role of these two carriers, GSH transport activity was enriched from rabbit kidney mitochondria and functionally reconstituted into phospholipid vesicles. Starting with 200 mg of mitoplast protein, 2 mg of partially enriched proteins were obtained after Triton X-114 solubilization and hydroxyapatite chromatography, The reconstituted proteoliposomes catalyzed butylmalonate-sensitive uptake of [C-14]malonate, phenylsuccinate-sensitive uptake of [C-14]2-oxoglutarate, and transport activity with [H-3]GSH. The initial rate of uptake of 5 mM GSH was approximately 170 nmol/min per mg protein, with a first-order rate constant of 0.3 min(-1), which is very close to that previously determined in freshly isolated rat kidney mitochondria. The enrichment procedure resulted in an approximately 60-fold increase in the specific activity of GSH transport, Substrates and inhibitors for the dicarboxylate and the a-oxoglutarate carriers (i.e,, malate, malonate, 2-oxoglutarate, butylmalonate, phenylsuccinate) significantly inhibited the uptake of [H-3]GSH, whereas most substrates for the tricarboxylate and monocarboxylate carriers had no effect. GSH uptake exhibited an apparent K-m of 2.8 mM and a V-max of 260 nmol/min per mg protein, Analysis of mutual inhibition between GSH and the dicarboxylates suggested that the dicarboxylate carrier contributes a somewhat higher proportion to overall GSH uptake and that both carriers account for 70 to 80% of total GSH uptake, These results provide further evidence for the function of the dicarboxylate and a-oxoglutarate carriers in the mitochondrial transport of GSH. (C) 2000 Academic Press [References: 32]
机译:在先前的研究中,我们提供了大鼠肾脏线粒体中二羧酸盐和α-氧代戊二酸酯载体吸收谷胱甘肽(GSH)的证据。为进一步研究这两种载体的作用,GSH转运活性从兔肾线粒体中富集并功能性重建进入磷脂囊泡。从200 mg的原生质体蛋白开始,经Triton X-114增溶和羟基磷灰石层析,获得2 mg部分富集的蛋白。重组蛋白脂质体催化丙二酸丁酯敏感的摄取,对[C- 14]丙二酸的丁二酸敏感的摄取。 14] 2-氧戊二酸酯,并具有[H-3] GSH的转运活性。最初摄取5 mM GSH的速率约为每毫克蛋白质170 nmol / min,一级速率常数为0.3 min(-1),与先前在新鲜分离的大鼠肾线粒体中测定的速率非常接近。富集程序导致GSH转运的比活性增加了约60倍,二羧酸盐和α-氧代戊二酸载体的底物和抑制剂(即苹果酸,丙二酸,2-氧代戊二酸,丙二酸丁酯,苯丁二酸)显着抑制了GSH转运。吸收[H-3] GSH,而大多数三羧酸盐和单羧酸盐载体的底物没有作用。 GSH吸收表现出2.8 KmM的表观Km和每毫克蛋白质260 nmol / min的V-max。对GSH和二羧酸盐之间的相互抑制作用的分析表明,二羧酸盐载体占总GSH摄入量的比例较高,并且两种载体占总GSH摄取的70%至80%。这些结果为二羧酸盐和α-氧代戊二酸酯载体在GSH线粒体运输中的功能提供了进一步的证据。 (C)2000年学术出版社[参考文献:32]

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