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首页> 外文期刊>The Journal of biological chemistry >Role of the Zn2+ Motif of E1 in SUMO Adenylation
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Role of the Zn2+ Motif of E1 in SUMO Adenylation

机译:e1 Zn2 +基序在Sumo腺苷酸中的作用

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Post-translational modifications by ubiquitin-like proteins are among the most important mechanisms for regulating a wide variety of cellular functions. In these modifications an E1 enzyme activates each ubiquitin-like protein (Ubl) by adenylation of the Ubl C-terminal COOH group and then forms a thioester bond with the adenylated C-terminal COOH group of the Ubl. Previous x-ray crystallography studies revealed a conserved zinc motif in the SUMO and NEDD8 E1; however, the function of this Zn2+ motif is unclear. In this study, using quantitative ATP:PPi isotope exchange assays in combination with site-directed mutagenesis, we show that the conserved Zn2+ motif in the SUMO E1 is important for SUMO adenylation and is critical for the E1 pseudo-ordered substrate binding mechanism. Furthermore, Zn2+ motif mutants showed significantly reduced kcat values for ATP:PPi isotope exchange assays, suggesting that the Zn2+ motif is important in binding and preventing SUMO adenylate from dissociating from E1 before formation of the thioester conjugate. Because the Zn2+ motif is located in a cross-over loop that is known to have conformational flexibility, the results described here suggest that this cross-over loop interacts with Ubl in the multistep, dynamic process of Ubl activation by E1s.
机译:泛素样蛋白的翻译后修饰是调节各种细胞功能的最重要机制之一。在这些修饰中,E1酶通过UBL C-末端COOH基团的腺苷化激活每个泛素样蛋白(UBL),然后与UBL的腺苷酸化C-末端COOH基团形成硫酯键。以前的X射线晶体学研究揭示了SUMO和NEDD8 E1中的保守锌基序;然而,该Zn2 +基序的功能尚不清楚。在该研究中,使用定量ATP:PPI同位素交换分析与点定向诱变,我们表明SUMO E1中的保守Zn2 +基序对于SuMo腺苷酸很重要,并且对于E1伪有序底物结合机制至关重要。此外,Zn2 +基序突变体显示出显着降低的ATP:PPI同位素交换测定的KCAT值,表明Zn2 +基序在结合和预防来自E1的结合和预防在形成硫酯缀合物之前的e1中的粘合剂。因为Zn2 +图案位于已知具有构象灵活性的交叉环中,所以这里描述的结果表明,这种交叉循环与UBL中的UBL中的UBL在E1S中的动态过程中相互作用。

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