DJ-1 可保护细胞免于因 GBA1 缺陷导致的线粒体氧化应激引起的细胞死亡。
DJ-1 protects cell death from a mitochondrial oxidative stress due to GBA1 deficiency.
机构信息
Department of Biology, Chungbuk National University, Cheongju, Chungbuk, 28644, Republic of Korea.
Department of Biological Sciences and Biotechnology, Chungbuk National University, Cheongju, Chungbuk, 28644, Republic of Korea.
出版信息
Genes Genomics. 2024 May;46(5):519-529. doi: 10.1007/s13258-024-01506-w. Epub 2024 Mar 9.
BACKGROUND
GBA1 mutations are the most common genetic risk factor for development of Parkinson's disease (PD). The loss of catalytic activity in GBA1, as well as the reduction of the GBA1 protein in certain cellular compartment, may increase disease progression. However, the mechanisms underlying cellular dysfunction caused by GBA1 deficiency are still mostly unknown.
OBJECTIVE
In this study, we focus on the genetic interaction between GBA1 deficiency and PD-causing genes, such as DJ-1, in mitochondrial dysfunction.
METHODS
GBA1 knockout (KO) SH-SY5Y cells were used to assess DJ-1 functions against oxidative stress in vitro. The levels of cellular reactive oxygen species were monitored with MitoSOX reagent. The expression of the PARK7 gene was analyzed using the quantitative real-time PCR (qRT-PCR). To understand the mechanism underlying DJ-1 upregulation in GBA1 KO cells, we assess ROS levels, antioxidant protein, and cell viability in GBA1 KO cells with treatment of ROS inhibitor N-acetyl-cysteine or miglustat, which is an inhibitor of glucosylceramide synthase. Dopaminergic degeneration was assessed from Gba1 L444P heterozygous mice mated with Park7 knockout mice.
RESULTS
We find that DJ-1 is significantly upregulated in GBA1 KO cells. Elevated levels of DJ-1 are attributed to the transcriptional expression of PARK7 mRNA, but not the inhibition of DJ-1 protein degradation. Because DJ-1 expression is highly linked to oxidative stress, we observe cellular reactive oxygen species (ROS) in GBA1 KO cells. Moreover, several antioxidant gene expressions and protein levels are increased in GBA1 KO cells. To this end, GBA1 KO cells are more susceptible to HO-induced cell death. Importantly, there is a significant reduction in dopaminergic neurons in the midbrain from Gba1 L444P heterozygous mice mated with Park7 knockout mice, followed by mild motor dysfunction.
CONCLUSION
Taken together, our results suggest that DJ-1 upregulation due to GBA1 deficiency has a protective role against oxidative stress. It may be supposed that mutations or malfunctions in the DJ-1 protein may have disadvantages in the survival of dopaminergic neurons in the brains of patients harboring GBA1 mutations.
背景
GBA1 突变是帕金森病 (PD) 发展的最常见遗传风险因素。GBA1 催化活性的丧失以及特定细胞区室中 GBA1 蛋白的减少,可能会增加疾病的进展。然而,GBA1 缺乏引起细胞功能障碍的机制在很大程度上仍不清楚。
目的
在这项研究中,我们专注于 GBA1 缺乏与 PD 致病基因(如 DJ-1)在线粒体功能障碍中遗传相互作用。
方法
使用 GBA1 敲除 (KO) SH-SY5Y 细胞体外评估 DJ-1 对氧化应激的作用。使用 MitoSOX 试剂监测细胞内活性氧的水平。使用定量实时 PCR (qRT-PCR) 分析 PARK7 基因的表达。为了了解 GBA1 KO 细胞中 DJ-1 上调的机制,我们评估了 GBA1 KO 细胞中 ROS 抑制剂 N-乙酰半胱氨酸或葡萄糖神经酰胺合酶抑制剂米格列醇处理后的 ROS 水平、抗氧化蛋白和细胞活力。从 Gba1 L444P 杂合子小鼠与 Park7 敲除小鼠交配的小鼠中评估多巴胺能神经元变性。
结果
我们发现 DJ-1 在 GBA1 KO 细胞中显著上调。DJ-1 水平升高归因于 PARK7 mRNA 的转录表达,而不是 DJ-1 蛋白降解的抑制。由于 DJ-1 表达与氧化应激高度相关,我们观察到 GBA1 KO 细胞中的细胞内活性氧 (ROS)。此外,GBA1 KO 细胞中的几种抗氧化基因表达和蛋白水平增加。为此,GBA1 KO 细胞对 HO 诱导的细胞死亡更敏感。重要的是,从 Gba1 L444P 杂合子小鼠与 Park7 敲除小鼠交配的小鼠的中脑中,多巴胺能神经元明显减少,随后出现轻度运动功能障碍。
结论
总之,我们的结果表明,由于 GBA1 缺乏导致的 DJ-1 上调具有对抗氧化应激的保护作用。可以假设,在携带 GBA1 突变的患者的大脑中,DJ-1 蛋白的突变或功能障碍可能对多巴胺能神经元的存活不利。
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