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使用化学合成的泛素和泛素化肽筛选泛素特异性蛋白酶活性。

Screening ubiquitin specific protease activities using chemically synthesized ubiquitin and ubiquitinated peptides.

作者信息

Bacchi Marine, Fould Benjamin, Jullian Magali, Kreiter Aude, Maurras Amélie, Nosjean Olivier, Coursindel Thibault, Puget Karine, Ferry Gilles, Boutin Jean A

机构信息

Pôle d'Expertise Biotechnologie, Chimie & Biologie, Institut de Recherches Servier, 125 Chemin de Ronde, 78290 Croissy-sur-Seine, France.

Genepep S.A., 12 Rue du Fer à Cheval, 34430 Saint-Jean-de-Védas, France.

出版信息

Anal Biochem. 2017 Feb 15;519:57-70. doi: 10.1016/j.ab.2016.12.014. Epub 2016 Dec 18.

DOI:10.1016/j.ab.2016.12.014
PMID:27993553
Abstract

Ubiquitin, a 76 amino acid protein, is a key component that contributes to cellular protein homeostasis. The specificity of this modification is due to a series of enzymes: ligases, attaching the ubiquitin to a lysine, and deubiquitinases, which remove it. More than a hundred of such proteins are implicated in the regulation of protein turnover. Their specificities are only partially understood. We chemically synthesized ubiquitin, attached it to lysines belonging to the protein sequences known to be ubiquitinated. We chose the model protein "murine double minute 2" (mdm2), a ubiquitin ligase, itself ubiquitinated and deubiquitinated. We folded the ubiquitinated peptides and checked their tridimensional conformation. We assessed the use of these substrates with a series of fifteen deubiquitinases to show the potentiality of such an enzymological technique. By manipulating the sequence of the peptide on which ubiquitin is attached, we were able to detect differences in the enzyme/substrate recognition, and to determine that these differences are deubiquitinase-dependent. This approach could be used to understand the substrate/protein relationship between the protagonists of this reaction. The methodology could be customized for a given substrate and used to advance our understanding of the key amino acids responsible for the deubiquitinase specificities.

摘要

泛素是一种由76个氨基酸组成的蛋白质,是维持细胞蛋白质稳态的关键成分。这种修饰的特异性归因于一系列酶:连接酶,将泛素连接到赖氨酸上;去泛素化酶,则负责去除泛素。一百多种此类蛋白质参与了蛋白质周转的调控。人们对它们的特异性只是部分了解。我们化学合成了泛素,并将其连接到已知会被泛素化的蛋白质序列的赖氨酸上。我们选择了模型蛋白“小鼠双微体2”(mdm2),一种泛素连接酶,其本身也会被泛素化和去泛素化。我们折叠了泛素化的肽段,并检查了它们的三维构象。我们用一系列十五种去泛素化酶评估了这些底物的使用情况,以展示这种酶学技术的潜力。通过操纵连接泛素的肽段序列,我们能够检测到酶/底物识别方面的差异,并确定这些差异是依赖于去泛素化酶的。这种方法可用于理解该反应中各主角之间的底物/蛋白质关系。该方法可针对给定底物进行定制,并用于加深我们对决定去泛素化酶特异性的关键氨基酸的理解。

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Screening ubiquitin specific protease activities using chemically synthesized ubiquitin and ubiquitinated peptides.使用化学合成的泛素和泛素化肽筛选泛素特异性蛋白酶活性。
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