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Structural basis of NEDD8 ubiquitin discrimination by the deNEDDylating enzyme NEDP1

机译:脱NEDDylating酶NEDP1鉴别NEDD8泛素的结构基础

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摘要

NEDD8 (neural precursor cell expressed developmentally downregulated gene 8)-specific protease NEDP1 processes preNEDD8 to its mature form and deconjugates NEDD8 from substrates such as p53 and cullins. Although NEDD8 and ubiquitin are highly related in sequence and structure, their attachment to a protein leads to different biological effects. It is therefore critical that NEDP1 discriminates between NEDD8 and ubiquitin, and this requires remarkable precision in molecular recognition. To determine the basis of this specificity, we have determined the crystal structure of NEDP1 in isolation and in a transition state complex with NEDD8. This reveals that NEDP1 is a cysteine protease of the Ulp family. Binding of NEDD8 induces a dramatic conformational change in a flexible loop that swings over the C-terminus of NEDD8 locking it into an extended β-structure optimal for catalysis. Structural, mutational and biochemical studies have identified key residues involved in molecular recognition. A single-residue difference in the C-terminus of NEDD8 and ubiquitin contributes significantly to the ability of NEDP1 to discriminate between them. In vivo analysis indicates that NEDP1 mutants perturb deNEDDylation of the tumour suppressor p53.
机译:NEDD8(神经前体细胞在发育中被下调的基因8表达)特异性蛋白酶NEDP1将preNEDD8加工成其成熟形式,并从p53和cullins等底物中解偶联NEDD8。尽管NEDD8和泛素在序列和结构上高度相关,但它们与蛋白质的附着会导致不同的生物学效应。因此,至关重要的是,NEDP1必须在NEDD8和泛素之间进行区分,这要求在分子识别中具有卓越的精确度。为了确定这种特异性的基础,我们确定了NEDP1的晶体结构,该晶体结构与NEDD8处于分离状态且处于过渡态。这表明NEDP1是Ulp家族的半胱氨酸蛋白酶。 NEDD8的结合在柔性环中引起剧烈的构象变化,该柔性环在NEDD8的C端上摇摆,将其锁定为最适合催化的扩展β结构。结构,突变和生化研究已确定了涉及分子识别的关键残基。 NEDD8和泛素C末端的单残基差异极大地促进了NEDP1区分它们的能力。体内分析表明,NEDP1突变体扰乱了肿瘤抑制因子p53的deNEDDylation。

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