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Biogenesis structure and function of the yeast 20S proteasome.

机译:酵母20S蛋白酶体的生物发生结构和功能。

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摘要

Intracellular degradation of many eukaryotic proteins requires their covalent ligation to ubiquitin. We previously identified a ubiquitin-dependent degradation pathway in the yeast Saccharomyces cerevisiae, the DOA pathway. Independent work has suggested that a major mechanism of cellular proteolysis involves a large multisubunit protease(s) called the 20S proteasome. We demonstrate here that Doa3 and Doa5, two essential components of the DOA pathway, are subunits of the proteasome. Biochemical analyses of purified mutant proteasomes suggest functions for several conserved proteasome subunit residues. All detectable proteasome particles purified from doa3 or doa5 cells have altered physical properties; however, the mutant particles contain the same 14 different subunits as the wild-type enzyme, indicating that most or all yeast 20S proteasomes comprise a uniform population of hetero-oligomeric complexes rather than a mixture of particles of variable subunit composition. Unexpectedly, we found that the yeast Doa3 and Pre3 subunits are synthesized as precursors which are processed in a manner apparently identical to that of related mammalian proteasome subunits implicated in antigen presentation, suggesting that biogenesis of the proteasome particle is highly conserved between yeast and mammals.
机译:许多真核蛋白质的细胞内降解需要它们与泛素共价连接。我们之前在酵母中发现了遍在蛋白依赖性降解途径,即DOA途径。独立研究表明,细胞蛋白水解的主要机制涉及一种称为20S蛋白酶体的大型多亚基蛋白酶。我们在这里证明Doa3和Doa5,DOA途径的两个基本组成部分,是蛋白酶体的亚基。纯化的突变体蛋白酶体的生化分析表明一些保守的蛋白酶体亚基残基的功能。从doa3或doa5细胞纯化的所有可检测的蛋白酶体颗粒均具有改变的物理特性;然而,突变体颗粒包含与野生型酶相同的14个不同的亚基,表明大多数或所有酵母20S蛋白酶体均包含均匀的异寡聚复合物群体,而不是可变亚基组成的颗粒混合物。出乎意料的是,我们发现酵母Doa3和Pre3亚基被合成为前体,其加工方式与涉及抗原呈递的相关哺乳动物蛋白酶体亚基的方式明显相同,这表明蛋白酶体颗粒的生物发生在酵母和哺乳动物之间高度保守。

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