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神经胶质纤维酸性蛋白的半胱氨酸残基是脂质过氧化作用的关键靶点,也是实现有效网络组织所必需的。

The cysteine residue of glial fibrillary acidic protein is a critical target for lipoxidation and required for efficient network organization.

机构信息

Department of Structural and Chemical Biology, Centro de Investigaciones Biológicas, C.S.I.C. Ramiro de Maeztu, 9, 28040 Madrid, Spain.

Laboratory of Astrocyte Biology and CNS Regeneration, Center for Brain Repair, Department of Clinical Neuroscience, Institute of Neuroscience and Physiology, Sahlgrenska Academy at the University of Gothenburg, Medicinaregatan 9 A, Gothenburg, Sweden.

出版信息

Free Radic Biol Med. 2018 May 20;120:380-394. doi: 10.1016/j.freeradbiomed.2018.04.007. Epub 2018 Apr 7.

DOI:10.1016/j.freeradbiomed.2018.04.007
PMID:29635011
Abstract

The type III intermediate filament protein glial fibrillary acidic protein (GFAP) contributes to the homeostasis of astrocytes, where it co-polymerizes with vimentin. Conversely, alterations in GFAP assembly or degradation cause intracellular aggregates linked to astrocyte dysfunction and neurological disease. Moreover, injury and inflammation elicit extensive GFAP organization and expression changes, which underline reactive gliosis. Here we have studied GFAP as a target for modification by electrophilic inflammatory mediators. We show that the GFAP cysteine, C294, is targeted by lipoxidation by cyclopentenone prostaglandins (cyPG) in vitro and in cells. Electrophilic modification of GFAP in cells leads to a striking filament rearrangement, with retraction from the cell periphery and juxtanuclear condensation in thick bundles. Importantly, the C294S mutant is resistant to cyPG addition and filament disruption, thus highlighting the critical role of this residue as a sensor of oxidative damage. However, GFAP C294S shows defective or delayed network formation in GFAP-deficient cells, including SW13/cl.2 cells and GFAP- and vimentin-deficient primary astrocytes. Moreover, GFAP C294S does not effectively integrate with and even disrupts vimentin filaments in the short-term. Interestingly, short-spacer bifunctional cysteine crosslinking produces GFAP-vimentin heterodimers, suggesting that a certain proportion of cysteine residues from both proteins are spatially close. Collectively, these results support that the conserved cysteine residue in type III intermediate filament proteins serves as an electrophilic stress sensor and structural element. Therefore, oxidative modifications of this cysteine could contribute to GFAP disruption or aggregation in pathological situations associated with oxidative or electrophilic stress.

摘要

III 型中间丝蛋白胶质纤维酸性蛋白 (GFAP) 与波形蛋白共聚合,有助于星形胶质细胞的内稳态。相反,GFAP 组装或降解的改变会导致与星形胶质细胞功能障碍和神经疾病相关的细胞内聚集物。此外,损伤和炎症会引起广泛的 GFAP 组织和表达变化,这突显了反应性神经胶质增生。在这里,我们研究了 GFAP 作为亲电炎症介质修饰的靶点。我们表明,环戊烯酮前列腺素 (cyPG) 在体外和细胞中靶向 GFAP 的半胱氨酸 C294 发生脂质过氧化。细胞中 GFAP 的亲电修饰导致明显的纤维重排,从细胞外周缩回,并在核周浓缩成厚束。重要的是,C294S 突变体对 cyPG 加合物和纤维破坏具有抗性,从而突出了该残基作为氧化损伤传感器的关键作用。然而,GFAP C294S 在包括 SW13/cl.2 细胞和 GFAP 和波形蛋白缺陷型原代星形胶质细胞在内的 GFAP 缺陷型细胞中显示出缺陷或延迟的网络形成。此外,GFAP C294S 不能有效地与波形蛋白纤维整合,甚至在短期内破坏波形蛋白纤维。有趣的是,短间隔双功能半胱氨酸交联产生 GFAP-波形蛋白异二聚体,表明两种蛋白质的某些比例的半胱氨酸残基在空间上接近。总之,这些结果支持 III 型中间丝蛋白中的保守半胱氨酸残基作为亲电应激传感器和结构元件。因此,这种半胱氨酸的氧化修饰可能导致与氧化或亲电应激相关的病理情况下 GFAP 的破坏或聚集。

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