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Dual function of Rpn5 in two PCI complexes, the 26S proteasome and COP9 signalosome

机译:Rpn5在两种PCI复合物26S蛋白酶体和COP9信号体中的双重功能

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Subunit composition and architectural structure of the 26S proteasome lid is strictly conserved between all eukaryotes. This eight-subunit complex bears high similarity to the eukaryotic translation initiation factor 3 and to the COP9 signalosome (CSN), which together define the proteasome CSN/COP9/initiation factor (PCI) troika. In some unicellular eukaryotes, the latter two complexes lack key subunits, encouraging questions about the conservation of their structural design. Here we demonstrate that, in Saccharomyces cerevisiae, Rpn5 plays dual roles by stabilizing proteasome and CSN structures independently. Proteasome and CSN complexes are easily dissected, with Rpn5 the only subunit in common. Together with Rpn5, we identified a total of six bona fide subunits at roughly stoichiometric ratios in isolated, affinity-purified CSN. Moreover, the copy of Rpn5 associated with the CSN is required for enzymatic hydrolysis of Rub1/Nedd8 conjugated to cullins. We propose that multitasking by a single subunit, Rpn5 in this case, allows it to function in different complexes simultaneously. These observations demonstrate that functional substitution of subunits by paralogues is feasible, implying that the canonical composition of the three PCI complexes in S.?cerevisiae is more robust than hitherto appreciated.
机译:所有真核生物之间都严格保留26S蛋白酶体盖的亚基组成和建筑结构。该八亚基复合物与真核翻译起始因子3和COP9信号小体(CSN)高度相似,后者共同定义了蛋白酶体CSN / COP9 /起始因子(PCI)三驾马车。在某些单细胞真核生物中,后两个复合物缺少关键的亚基,这引发了有关其结构设计保守性的问题。在这里,我们证明,在酿酒酵母中,Rpn5通过独立稳定蛋白酶体和CSN结构发挥双重作用。蛋白酶体和CSN复合物很容易分解,其中Rpn5是唯一的共同亚基。我们与Rpn5一起,在分离的,亲和纯化的CSN中以大致化学计量比鉴定了总共六个真正的亚基。此外,与CSN缔合的Rpn5的拷贝是酶水解与cullins结合的Rub1 / Nedd8所必需的。我们建议通过单个子单元Rpn5进行多任务处理,在这种情况下,它可以同时在不同的复合体中运行。这些观察结果表明,通过旁系同源物进行亚基的功能取代是可行的,这意味着酿酒酵母中三个PCI复合物的规范组成比迄今所认可的更牢固。

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