过量的同型半胱氨酸上调视网膜 Müller 胶质细胞中的 NRF2 抗氧化途径。
Excess homocysteine upregulates the NRF2-antioxidant pathway in retinal Müller glial cells.
机构信息
Department of Cellular Biology and Anatomy, Medical College of Georgia, Augusta University, Augusta, GA, United States; James and Jean Culver Vision Discovery Institute, Augusta University, Augusta, GA, United States.
Department of Pharmacology and Toxicology, Medical College of Georgia, Augusta University, Augusta, GA, United States.
出版信息
Exp Eye Res. 2019 Jan;178:228-237. doi: 10.1016/j.exer.2018.03.022. Epub 2018 Mar 31.
This study evaluated the effects of elevated homocysteine (Hcy) on the oxidative stress response in retinal Müller glial cells. Elevated Hcy has been implicated in retinal diseases including glaucoma and optic neuropathy, which are characterized by retinal ganglion cell (RGC) loss. To understand the mechanisms of Hcy-induced RGC loss, in vitro and in vivo models have been utilized. In vitro isolated RGCs are quite sensitive to elevated Hcy levels, while in vivo murine models of hyperhomocysteinemia (HHcy) demonstrate a more modest RGC loss (∼20%) over a period of many months. This differential response to Hcy between isolated cells and the intact retina suggests that the retinal milieu invokes mechanisms that buffer excess Hcy. Oxidative stress has been implicated as a mechanism of Hcy-induced neuron loss and NRF2 is a transcription factor that plays a major role in regulating cytoprotective responses to oxidative stress. In the present study we investigated whether HHcy upregulates NRF2-mediated stress responses in Müller cells, the chief retinal glial cell responsible for providing trophic support to retinal neurons. Primary Müller cells were exposed to L-Hcy-thiolactone [50μM-10mM] and assessed for viability, reactive oxygen species (ROS), and glutathione (GSH) levels. Gene/protein levels of Nrf2 and levels of NRF2-regulated antioxidants (NQO1, CAT, SOD2, HMOX1, GPX1) were assessed in Hcy-exposed Müller cells. Unlike isolated RGCs, isolated Müller cells are viable over a wide range of Hcy concentrations [50 μM - 1 mM]. Moreover, when exposed to elevated Hcy, Müller cells demonstrate decreased oxidative stress and decreased ROS levels. GSH levels increased by ∼20% within 24 h exposure to Hcy. Molecular analyses revealed 2-fold increase in Nrf2 expression. Expression of antioxidant genes Nqo1, Cat, Sod2, Hmox1, Gpx1 increased significantly. The consequences of Hcy exposure were evaluated also in Müller cells harvested from Nrf2 mice. In contrast to WT Müller cells, in which oxidative stress decreased upon exposure to Hcy, the Nrf2 Müller cells showed a significant increase in oxidative stress. Our data suggest that at least during early stages of Hhcy, a cytoprotective response may be in place, mediated in part by NRF2 in Müller cells.
本研究评估了高同型半胱氨酸(Hcy)对视网膜 Müller 胶质细胞氧化应激反应的影响。高 Hcy 与包括青光眼和视神经病变在内的视网膜疾病有关,这些疾病的特征是视网膜神经节细胞(RGC)丢失。为了了解 Hcy 诱导的 RGC 丢失的机制,已利用体外和体内模型。体外分离的 RGC 对高 Hcy 水平非常敏感,而在高同型半胱氨酸血症(HHcy)的体内小鼠模型中,在数月的时间内仅观察到约 20%的 RGC 丢失。这种分离细胞与完整视网膜对 Hcy 的反应差异表明,视网膜环境引发了缓冲多余 Hcy 的机制。氧化应激已被认为是 Hcy 诱导神经元丢失的机制,而 NRF2 是一种转录因子,在调节对氧化应激的细胞保护反应中起主要作用。在本研究中,我们研究了 HHcy 是否会上调 Müller 细胞中 NRF2 介导的应激反应,Müller 细胞是负责向视网膜神经元提供营养支持的主要视网膜神经胶质细胞。将原代 Müller 细胞暴露于 L-Hcy-硫内酯[50μM-10mM]中,并评估其活力、活性氧(ROS)和谷胱甘肽(GSH)水平。在 Hcy 暴露的 Müller 细胞中评估 Nrf2 的基因/蛋白水平和 NRF2 调节的抗氧化剂(NQO1、CAT、SOD2、HMOX1、GPX1)水平。与分离的 RGC 不同,分离的 Müller 细胞在广泛的 Hcy 浓度[50μM-1mM]下保持活力。此外,当暴露于高 Hcy 时,Müller 细胞表现出氧化应激和 ROS 水平降低。在 24 小时暴露于 Hcy 后,GSH 水平增加了约 20%。分子分析显示 Nrf2 表达增加了 2 倍。抗氧化基因 Nqo1、Cat、Sod2、Hmox1、Gpx1 的表达显著增加。还在来自 Nrf2 小鼠的 Müller 细胞中评估了 Hcy 暴露的后果。与在 Hcy 暴露下氧化应激降低的 WT Müller 细胞相反,Nrf2 Müller 细胞的氧化应激显著增加。我们的数据表明,至少在 HHcy 的早期阶段,可能存在一种细胞保护反应,部分由 Müller 细胞中的 NRF2 介导。
Zotero 插件