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用于泛素的双E1激活系统对E2酶负载进行差异调节。

Dual E1 activation systems for ubiquitin differentially regulate E2 enzyme charging.

作者信息

Jin Jianping, Li Xue, Gygi Steven P, Harper J Wade

机构信息

Department of Pathology, Harvard Medical School, 77 Avenue Louis Pasteur, Boston, Massachusetts 02115, USA.

出版信息

Nature. 2007 Jun 28;447(7148):1135-8. doi: 10.1038/nature05902.

Abstract

Modification of proteins with ubiquitin or ubiquitin-like proteins (UBLs) by means of an E1-E2-E3 cascade controls many signalling networks. Ubiquitin conjugation involves adenylation and thioesterification of the carboxy-terminal carboxylate of ubiquitin by the E1-activating enzyme Ube1 (Uba1 in yeast), followed by ubiquitin transfer to an E2-conjugating enzyme through a transthiolation reaction. Charged E2s function with E3s to ubiquitinate substrates. It is currently thought that Ube1/Uba1 is the sole E1 for charging of E2s with ubiquitin in animals and fungi. Here we identify a divergent E1 in vertebrates and sea urchin, Uba6, which specifically activates ubiquitin but not other UBLs in vitro and in vivo. Human Uba6 and Ube1 have distinct preferences for E2 charging in vitro, and their specificity depends in part on their C-terminal ubiquitin-fold domains, which recruit E2s. In tissue culture cells, Uba6 is required for charging a previously uncharacterized Uba6-specific E2 (Use1), whereas Ube1 is required for charging the cell-cycle E2s Cdc34A and Cdc34B. Our data reveal unexpected complexity in the pathways that control the conjugation of ubiquitin, in which dual E1s orchestrate the charging of distinct cohorts of E2s.

摘要

通过E1-E2-E3级联反应将泛素或类泛素蛋白(UBLs)与蛋白质进行修饰,可控制许多信号网络。泛素缀合涉及泛素的羧基末端羧酸盐通过E1激活酶Ube1(酵母中的Uba1)进行腺苷酸化和硫酯化,随后通过转硫醇反应将泛素转移至E2缀合酶。带电荷的E2与E3共同作用使底物泛素化。目前认为,Ube1/Uba1是动物和真菌中唯一用于使E2与泛素结合的E1。在此,我们在脊椎动物和海胆中鉴定出一种不同的E1,即Uba6,其在体外和体内特异性激活泛素而非其他UBLs。人Uba6和Ube1在体外对E2结合具有不同偏好,其特异性部分取决于招募E2的C末端泛素折叠结构域。在组织培养细胞中,使先前未表征的Uba6特异性E2(Use1)结合需要Uba6,而使细胞周期E2s Cdc34A和Cdc34B结合需要Ube1。我们的数据揭示了控制泛素缀合途径中意想不到的复杂性,其中双E1协调不同E2群体的结合。

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