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Total Chemical Synthesis of SUMO and SUMO-Based Probes for Profiling the Activity of SUMO-Specific Proteases

机译:总结基于SUMO和SUMO的探针的总化学合成,用于分析SUMO特异性蛋白酶的活性

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摘要

SUMO is a post-translational modifier critical for cell cycle progression and genome stability that plays a role in tumorigenesis, thus rendering SUMO-specific enzymes potential pharmacological targets. However, the systematic generation of tools for the activity profiling of SUMO-specific enzymes has proven challenging. We developed a diversifiable synthetic platform for SUMO-based probes by using a direct linear synthesis method, which permits N- and C-terminal labelling to incorporate dyes and reactive warheads, respectively. In this manner, activity-based probes (ABPs) for SUMO-1, SUMO-2, and SUMO-3-specific proteases were generated and validated in cells using gel-based assays and confocal microscopy. We further expanded our toolbox with the synthesis of a K11-linked diSUMO-2 probe to study the proteolytic cleavage of SUMO chains. Together, these ABPs demonstrate the versatility and specificity of our synthetic SUMO platform for invitro and invivo characterization of the SUMO protease family.
机译:SUMO是一种翻译后改性剂,适用于在肿瘤发生中发挥作用的细胞周期进展和基因组稳定性,从而使SUMO特异性酶潜在的药理学靶标。然而,SUMO特异性酶活性分析的系统产生的工具已经证明了具有挑战性。我们通过使用直接线性合成方法开发了一种用于基于SUMO的探针的多元化合成平台,其允许N-和C末端标记分别包含染料和活性弹头。以这种方式,使用基于凝胶的测定和共聚焦显微镜在细胞中产生并验证SUMO-1,SUMO-2和SUMO-3特异性蛋白酶的基于活性的探针(ABP)。我们进一步扩展了我们的工具箱,合成了K11链接的DISOM-2探针,研究了Sumo链的蛋白水解裂解。这些ABPS一起证明了我们合成的Sumo平台的通用性和特异性Sumo蛋白酶家族的Invitro和Invivo表征。

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