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酒精驱动蛋白磷酸酶1的亚硝基化和氧化还原激活,导致牛气道纤毛功能障碍。

Alcohol drives -nitrosylation and redox activation of protein phosphatase 1, causing bovine airway cilia dysfunction.

作者信息

Price Michael E, Pavlik Jacqueline A, Liu Miao, Ding Shi-Jian, Wyatt Todd A, Sisson Joseph H

机构信息

Pulmonary, Critical Care, Sleep and Allergy Division, Department of Internal Medicine, University of Nebraska Medical Center, Omaha, Nebraska.

Department of Cellular and Integrative Physiology, University of Nebraska Medical Center, Omaha, Nebraska.

出版信息

Am J Physiol Lung Cell Mol Physiol. 2017 Mar 1;312(3):L432-L439. doi: 10.1152/ajplung.00513.2016. Epub 2017 Jan 6.

Abstract

Individuals with alcohol (ethanol)-use disorders are at increased risk for lung infections, in part, due to defective mucociliary clearance driven by motile cilia in the airways. We recently reported that isolated, demembranated bovine cilia (axonemes) are capable of producing nitric oxide (NO) when exposed to biologically relevant concentrations of alcohol. This increased presence of NO can lead to protein -nitrosylation, a posttranslational modification signaling mechanism involving reversible adduction of nitrosonium cations or NO to thiolate or thiyl radicals, respectively, of proteins forming -nitrosothiols (SNOs). We quantified and compared SNO content between isolated, demembranated axonemes extracted from bovine tracheae, with or without in situ alcohol exposure (100 mM × 24 h). We demonstrate that relevant concentrations of alcohol exposure shift the -nitrosylation status of key cilia regulatory proteins, including 20-fold increases in -nitrosylation of proteins that include protein phosphatase 1 (PP1). With the use of an ATP-reactivated axoneme motility system, we demonstrate that alcohol-driven -nitrosylation of PP1 is associated with PP1 activation and dysfunction of axoneme motility. These new data demonstrate that alcohol can shift the -nitrothiol balance at the level of the cilia organelle and highlight -nitrosylation as a novel signaling mechanism to regulate PP1 and cilia motility.

摘要

患有酒精(乙醇)使用障碍的个体肺部感染风险增加,部分原因是气道中活动纤毛驱动的黏液纤毛清除功能存在缺陷。我们最近报告称,分离的、去膜的牛纤毛(轴丝)在暴露于生物学相关浓度的酒精时能够产生一氧化氮(NO)。NO的这种增加会导致蛋白质亚硝基化,这是一种翻译后修饰信号机制,分别涉及硝鎓阳离子或NO与蛋白质的硫醇盐或硫基自由基可逆加成,形成亚硝基硫醇(SNOs)。我们对从牛气管中提取的分离的、去膜的轴丝进行原位酒精暴露(100 mM×24小时)或不暴露的情况下的SNO含量进行了定量和比较。我们证明,相关浓度的酒精暴露会改变关键纤毛调节蛋白的亚硝基化状态,包括蛋白磷酸酶1(PP1)等蛋白质的亚硝基化增加20倍。通过使用ATP激活的轴丝运动系统,我们证明酒精驱动的PP1亚硝基化与PP1激活和轴丝运动功能障碍有关。这些新数据表明,酒精可以在纤毛细胞器水平上改变亚硝基硫醇平衡,并突出亚硝基化作为调节PP1和纤毛运动的一种新的信号机制。

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引用本文的文献

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本文引用的文献

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Am J Physiol Lung Cell Mol Physiol. 2015 Mar 15;308(6):L577-85. doi: 10.1152/ajplung.00336.2014. Epub 2015 Jan 9.
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