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Chemical-proteomic strategies to investigate cysteine posttranslational modifications

机译:化学蛋白质组学策略研究半胱氨酸翻译后修饰

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摘要

The unique combination of nucleophilicity and redox-sensitivity that is characteristic of cysteine residues results in a variety of posttranslational modifications (PTMs), including oxidation, nitrosation, glutathionylation, prenylation, palmitoylation and Michael adducts with lipid-derived electrophiles (LDEs). These PTMs regulate the activity of diverse protein families by modulating the reactivity of cysteine nucleophiles within active sites of enzymes, and governing protein localization between soluble and membrane-bound forms. Many of these modifications are highly labile, sensitive to small changes in the environment, and dynamic, rendering it difficult to detect these modified species within a complex proteome. Several chemical-proteomic platforms have evolved to study these modifications and enable a better understanding of the diversity of proteins that are regulated by cysteine PTMs. These platforms include: (1) chemical probes to selectively tag PTM-modified cysteines; (2) differential labeling platforms that selectively reveal and tag PTM-modified cysteines; (3) lipid, isoprene and LDE derivatives containing bioorthogonal handles; and (4) cysteine-reactivity profiling to identify PTM-induced decreases in cysteine nucleophilicity. Here, we will provide an overview of these existing chemical-proteomic strategies and their effectiveness at identifying PTM-modified cysteine residues within native biological systems.
机译:半胱氨酸残基所特有的亲核性和氧化还原敏感性的独特结合导致了各种翻译后修饰(PTM),包括氧化,亚硝化,谷胱甘肽化,戊烯化,棕榈酰化和与脂质衍生的亲电试剂(LDE)的迈克尔加成反应。这些PTM通过调节酶活性位点内的半胱氨酸亲核试剂的反应性,并控制可溶性和膜结合形式之间的蛋白质定位,从而调节各种蛋白质家族的活性。这些修饰中的许多修饰非常不稳定,对环境的微小变化敏感,并且动态变化,因此很难在复杂的蛋白质组中检测到这些修饰的物种。已经开发出了几种化学蛋白质组学平台来研究这些修饰,并能够更好地了解由半胱氨酸PTM调节的蛋白质的多样性。这些平台包括:(1)用于选择性标记PTM修饰的半胱氨酸的化学探针; (2)选择性标记平台,选择性地揭示和标记经PTM修饰的半胱氨酸; (3)含有生物正交柄的脂质,异戊二烯和LDE衍生物; (4)半胱氨酸反应性分析,以鉴定PTM诱导的半胱氨酸亲核性降低。在这里,我们将概述这些现有的化学蛋白质组学策略及其在天然生物系统中鉴定PTM修饰的半胱氨酸残基的有效性。

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