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Protein synthesis by brain-cortex mitochondria. Characterization of a 55S mitochondrial ribosome as the functional unit in protein synthesis by cortex mitochondria and its distinction from a contaminant cytoplasmic protein-synthesizing system

机译:大脑皮质线粒体的蛋白质合成。 55S线粒体核糖体作为皮层线粒体蛋白质合成中的功能单元的表征及其与污染物胞质蛋白质合成系统的区别

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摘要

Homogenates of rat brain cortex were fractionated by conventional methods of velocity sedimentation and separated into a microsomal and a washed mitochondrial fraction. By electron microscopy the mitochondrial fraction was shown to be rich in synaptosomes. The mitochondria–synaptosome fraction synthesized protein in vitro by a route that was partially inhibited by cycloheximide and partly by chloramphenicol. The relative effectiveness of the two inhibitors varied greatly with the medium used. In the mitochondria–synaptosome fraction active 80S cytoplasmic ribosomes and active 55S mitochondrial ribosomes were detected; these were also seen in the electron microscope. Mild osmotic shock of the mitochondria–synaptosome fraction followed by velocity sedimentation in sucrose–EDTA allowed isolation of a mitochondrial fraction free of synaptosomes. Protein synthesis in this fraction was entirely inhibited by chloramphenicol, but was completely resistant to cycloheximide both in a medium promoting oxidative phosphorylation and in ATP-generating medium. Ouabain had no inhibitory effect on protein synthesis in a purified mitochondrial preparation. It is concluded that brain-cortex mitochondria synthesize protein entirely on 55S mitochondrial ribosomes.
机译:用常规的速度沉降方法将大鼠大脑皮层的匀浆物分级,分成微粒体和洗涤过的线粒体级分。通过电子显微镜观察,线粒体部分富含突触小体。线粒体-突触体部分在体外通过部分被环己酰亚胺抑制,部分被氯霉素抑制的途径合成蛋白质。两种抑制剂的相对效力随所用培养基的不同而有很大差异。在线粒体-突触体部分中检测到了活跃的80S胞质核糖体和活跃的55S线粒体核糖体。这些在电子显微镜下也可以看到。线粒体-突触体部分的轻度渗透性休克,然后在蔗糖-EDTA中进行速度沉降,从而可以分离出不含突触体的线粒体部分。该级分中的蛋白质合成被氯霉素完全抑制,但在促进氧化磷酸化的介质和在产生ATP的介质中都完全抗环己酰亚胺。哇巴因对纯化的线粒体制剂中的蛋白质合成没有抑制作用。结论是脑皮质线粒体完全在55S线粒体核糖体上合成蛋白质。

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