Thioether-mediated protein ubiquitination in constructing affinity- and activity-based ubiquitinated protein probes.

IF 13.1 1区生物学 Q1 BIOCHEMICAL RESEARCH METHODS

Nature Protocols Pub Date : 2025-04-25 DOI:10.1038/s41596-025-01162-8

Gregory A Davidson, Zeinab Moafian, Amanda R Sensi, Zhihao Zhuang

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引用次数: 0

Abstract

Protein ubiquitination, a critical regulatory mechanism and post-translational modification in eukaryotic cells, involves the formation of an isopeptide bond between ubiquitin (Ub) and targeted proteins. Despite extensive investigation into the roles played by protein ubiquitination in various cellular processes, many questions remain to be answered. A major challenge in the biochemical and biophysical characterization of protein ubiquitination, along with its associated pathways and protein players, lies in the generation of ubiquitinated proteins, either in mono- or poly-ubiquitinated forms. Enzymatic and chemical strategies have been reported to address this challenge; however, there are still unmet needs for the facile generation of ubiquitinated proteins in the quantity and homogeneity required to precisely decipher the role of various protein-specific ubiquitination events. In this protocol, we provide the ubiquitin research community with a chemical ubiquitination method enabled by an α-bromoketone-mediated ligation strategy. This method can be readily adapted to generate mono- and poly-ubiquitinated proteins of interest through a cysteine introduced to replace the target lysine, with the native cysteines mutated to serine. Using proliferating cell nuclear antigen (PCNA) as an example, we present herein a detailed protocol for generating di- and tri-Ub PCNA that contains a photo-activatable cross-linker for capturing potential reader proteins. The thioether-mediated protein ligation and purification typically takes 2-3 weeks. An important feature of our ubiquitination strategy is the ability to introduce a Michael-acceptor warhead to the linkage, allowing the generation of activity-based probes for deubiquitinases and ubiquitin-carrying enzymes such as HECT and RBR E3 ubiquitin ligases and E2 enzymes. As such, our method is highly versatile and can be readily adapted to investigate the readers and erasers of many proteins that undergo reversible ubiquitination.

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构建基于亲和和活性的泛素化蛋白探针的硫醚介导的蛋白质泛素化。

蛋白质泛素化是真核细胞中一个重要的调控机制和翻译后修饰，涉及泛素（Ub）与靶蛋白之间形成异肽键。尽管对蛋白质泛素化在各种细胞过程中所起的作用进行了广泛的研究，但仍有许多问题有待解答。蛋白质泛素化及其相关途径和蛋白质参与者的生化和生物物理特征的主要挑战在于泛素化蛋白的产生，无论是单泛素化还是多泛素化形式。据报道，酶和化学策略可以解决这一挑战；然而，对于泛素化蛋白的快速生成，在数量和均匀性上仍然没有得到满足，这需要精确地破译各种蛋白质特异性泛素化事件的作用。在本协议中，我们为泛素研究界提供了一种由α-溴酮介导的连接策略激活的化学泛素化方法。这种方法可以很容易地适应于产生感兴趣的单和多泛素化蛋白，通过引入半胱氨酸来取代目标赖氨酸，使天然半胱氨酸突变为丝氨酸。以增殖细胞核抗原（PCNA）为例，我们在这里提出了一个详细的方案，以产生含有光激活交联剂的二和三ub PCNA，用于捕获潜在的读取器蛋白。硫醚介导的蛋白连接和纯化通常需要2-3周。我们的泛素化策略的一个重要特点是能够将michael -受体战斗部引入到链接中，从而可以生成基于活性的探针，用于脱泛素酶和泛素携带酶，如HECT和RBR E3泛素连接酶和E2酶。因此，我们的方法是高度通用的，可以很容易地适应于研究许多经历可逆泛素化的蛋白质的读取器和擦除器。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Nature Protocols 生物-生化研究方法

CiteScore

29.10

自引率

0.70%

发文量

128

审稿时长

4 months

期刊介绍： Nature Protocols focuses on publishing protocols used to address significant biological and biomedical science research questions, including methods grounded in physics and chemistry with practical applications to biological problems. The journal caters to a primary audience of research scientists and, as such, exclusively publishes protocols with research applications. Protocols primarily aimed at influencing patient management and treatment decisions are not featured. The specific techniques covered encompass a wide range, including but not limited to: Biochemistry, Cell biology, Cell culture, Chemical modification, Computational biology, Developmental biology, Epigenomics, Genetic analysis, Genetic modification, Genomics, Imaging, Immunology, Isolation, purification, and separation, Lipidomics, Metabolomics, Microbiology, Model organisms, Nanotechnology, Neuroscience, Nucleic-acid-based molecular biology, Pharmacology, Plant biology, Protein analysis, Proteomics, Spectroscopy, Structural biology, Synthetic chemistry, Tissue culture, Toxicology, and Virology.