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The structure of SENP1–SUMO-2 complex suggests a structural basis for discrimination between SUMO paralogues during processing

机译:SENP1–SUMO-2复合物的结构为加工过程中SUMO旁系同源物之间的区分提供了结构基础

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pThe SUMO (small ubiquitin-like modifier)-specific protease SENP1 (sentrin-specific protease 1) can process the three forms of SUMO to their mature forms and deconjugate SUMO from modified substrates. It has been demonstrated previously that SENP1 processed SUMO-1 more efficiently than SUMO-2, but displayed little difference in its ability to deconjugate the different SUMO paralogues from modified substrates. To determine the basis for this substrate specificity, we have determined the crystal structure of SENP1 in isolation and in a transition-state complex with SUMO-2. The interface between SUMO-2 and SENP1 has a relatively poor complementarity, and most of the recognition is determined by interaction between the conserved C-terminus of SUMO-2 and the cleft in the protease. Although SENP1 is rather similar in structure to the related protease SENP2, these proteases have different SUMO-processing activities. Electrostatic analysis of SENP1 in the region where the C-terminal peptide, removed during maturation, would project indicates that it is the electrostatic complementarity between this region of SENP1 and the C-terminal peptides of the various SUMO paralogues that mediates selectivity./p
机译:> SUMO(小泛素样修饰剂)特异性蛋白酶SENP1(Sentrin特异性蛋白酶1)可以将SUMO的三种形式加工成它们的成熟形式,并从修饰的底物中解偶联SUMO。先前已经证明SENP1比SUMO-2更有效地处理SUMO-1,但是在其从修饰的底物上解偶联不同SUMO旁系同源物的能力上显示出很小的差异。为了确定这种底物特异性的基础,我们已经确定了SENP1的晶体结构,该晶体结构是与SUMO-2分离且处于过渡态复合物。 SUMO-2和SENP1之间的界面具有相对较弱的互补性,并且大多数识别是由SUMO-2的保守C末端与蛋白酶中的裂口之间的相互作用决定的。尽管SENP1在结构上与相关的蛋白酶SENP2相似,但这些蛋白酶具有不同的SUMO加工活性。预测在成熟过程中C末端肽被去除的区域中SENP1的静电分析表明,SENP1的该区域与各种SUMO旁系同源物的C末端肽之间的静电互补决定了选择性。

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