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蛋白酶体α7同型十四聚体的自组装双环结构被α6拆解。

Disassembly of the self-assembled, double-ring structure of proteasome α7 homo-tetradecamer by α6.

作者信息

Ishii Kentaro, Noda Masanori, Yagi Hirokazu, Thammaporn Ratsupa, Seetaha Supaporn, Satoh Tadashi, Kato Koichi, Uchiyama Susumu

机构信息

Okazaki Institute for Integrative Bioscience, National Institutes of Natural Sciences, 5-1 Higashiyama, Myodaiji, Okazaki, Aichi 444-8787, Japan.

Department of Biotechnology, Graduate School of Engineering, Osaka University, 2-1 Yamadaoka, Suita, Osaka 565-0871, Japan.

出版信息

Sci Rep. 2015 Dec 14;5:18167. doi: 10.1038/srep18167.

Abstract

The 20S core particle of the eukaryotic proteasome is composed of two α- and two β-rings, each of which is a hetero-heptamer composed of seven homologous but distinct subunits. Although formation of the eukaryotic proteasome is a highly ordered process assisted by assembly chaperones, α7, an α-ring component, has the unique property of self-assembling into a homo-tetradecamer. We used biophysical methods to characterize the oligomeric states of this proteasome subunit and its interaction with α6, which makes direct contacts with α7 in the proteasome α-ring. We determined a crystal structure of the α7 tetradecamer, which has a double-ring structure. Sedimentation velocity analytical ultracentrifugation and mass spectrometric analysis under non-denaturing conditions revealed that α7 exclusively exists as homo-tetradecamer in solution and that its double-ring structure is disassembled upon the addition of α6, resulting in a 1:7 hetero-octameric α6-α7 complex. Our findings suggest that proteasome formation involves the disassembly of non-native oligomers, which are assembly intermediates.

摘要

真核生物蛋白酶体的20S核心颗粒由两个α环和两个β环组成,每个环都是由七个同源但不同的亚基组成的异源七聚体。尽管真核生物蛋白酶体的形成是一个由组装伴侣辅助的高度有序的过程,但α环成分α7具有自组装成同型十四聚体的独特性质。我们使用生物物理方法来表征该蛋白酶体亚基的寡聚状态及其与α6的相互作用,α6在蛋白酶体α环中与α7直接接触。我们确定了α7十四聚体的晶体结构,其具有双环结构。非变性条件下的沉降速度分析超速离心和质谱分析表明,α7在溶液中仅以同型十四聚体形式存在,并且在添加α6后其双环结构会解体,形成1:7的异源八聚体α6-α7复合物。我们的研究结果表明,蛋白酶体的形成涉及非天然寡聚体的解体,这些非天然寡聚体是组装中间体。

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