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一氧化氮通过控制氧的可利用性促进半胱氨酸N-端规则途径的蛋白质水解。

Nitric oxide promotes cysteine N-degron proteolysis through control of oxygen availability.

作者信息

Kim Haeun, Tian Ya-Min, Ratcliffe Peter J, Keeley Thomas P

机构信息

Target Discovery Institute, Nuffield Department of Medicine, University of Oxford, Oxford OX3 7FZ, United Kingdom.

Ludwig Institute for Cancer Research, Nuffield Department of Medicine, University of Oxford, Oxford OX3 7DQ, United Kingdom.

出版信息

Proc Natl Acad Sci U S A. 2025 Aug 26;122(34):e2501796122. doi: 10.1073/pnas.2501796122. Epub 2025 Aug 19.

DOI:10.1073/pnas.2501796122
PMID:40828020
Abstract

Selected proteins containing an N-terminal cysteine (Nt-Cys) are subjected to rapid, O-dependent proteolysis via the Cys/Arg-branch of the N-degron pathway. Cysteine dioxygenation is catalyzed in mammalian cells by 2-aminoethanethiol dioxygenase (ADO), an enzyme that manifests extreme O sensitivity. The canonical substrates of this pathway in mammalia are the regulators of G-protein signaling 4, 5, and 16, as well as interleukin-32. In addition to operating as an O-sensing mechanism, this pathway has previously been described as a sensor of nitric oxide (NO), with robust effects on substrate stability upon modulation of NO bioavailability being widely demonstrated. Despite this, no mechanism to describe the action of NO on the Cys/Arg N-degron pathway has yet been substantiated. We demonstrate that NO can regulate the stability of Cys N-degron substrates indirectly via the regulation of ADO cosubstrate availability. Through competitive, O-dependent inhibition of cytochrome C oxidase, NO can substantially modify cellular O consumption rate and, in doing so, alter the availability of O for Nt-Cys dioxygenation. We show that this increase in O availability in response to NO exposure is sufficient to alter both dynamic and steady-state ADO substrate levels. It is likely that this mechanism operates to couple O supply and mitochondrial respiration with responses to G-protein-coupled receptor stimulation.

摘要

含有N端半胱氨酸(Nt-Cys)的特定蛋白质会通过N-降解子途径的半胱氨酸/精氨酸分支,经历快速的、氧依赖性蛋白水解。在哺乳动物细胞中,半胱氨酸双加氧作用由2-氨基乙硫醇双加氧酶(ADO)催化,该酶对氧表现出极高的敏感性。在哺乳动物中,此途径的典型底物是G蛋白信号调节因子4、5和16,以及白细胞介素-32。除了作为一种氧感应机制外,该途径此前还被描述为一种一氧化氮(NO)传感器,广泛证明了调节NO生物利用度对底物稳定性有显著影响。尽管如此,尚未证实描述NO对半胱氨酸/精氨酸N-降解子途径作用的机制。我们证明,NO可通过调节ADO共底物的可用性间接调节半胱氨酸N-降解子底物的稳定性。通过对细胞色素C氧化酶的竞争性、氧依赖性抑制,NO可显著改变细胞的氧消耗率,并由此改变用于Nt-Cys双加氧作用的氧的可用性。我们表明,这种因暴露于NO而导致的氧可用性增加足以改变动态和稳态的ADO底物水平。这种机制可能用于将氧供应和线粒体呼吸与对G蛋白偶联受体刺激的反应联系起来。

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