Rui-han Liu , Xing-chen Wang , Yu Kong , Xiang-yu Xiao , Ting Sun , Qiu-bo Li , Qing-xia Kong
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引用次数: 0
Abstract
Background
Drug-resistant epilepsy (DRE) affects more than 20 million people worldwide. DRE patients do not respond to anti-seizure medications. Shifting from anti-seizure to anti-epileptic and disease-modifying therapy will be an important aim for future research. The canonical nuclear factor kappa B (NF-κB) signaling pathway plays a pivotal role in epilepsy and neuroinflammation. However, the expression and regulation of RelB, which can be activated via both canonical and non-canonical NF-κB signaling, are obscure in epilepsy. To clarify the expression and localization of RelB in the DRE phenotype and to determine the proteins related to RelB regulation, we conducted the following studies.
Methods
Quantitative PCR was performed to detect the transcription of RELB in pilocarpine-induced epileptic rats. Western blotting was used to determine the abundance of RelB and proteins related to RelB regulation in brain tissue from both epilepsy model rats and DRE patients and in liposaccharide-induced HT22 cells. Immunofluorescence staining and immunohistochemistry were used to locate RelB in brain sections from DRE patients. ELISA was used to determine inflammatory cytokines secreted by HT22 cells into the culture medium.
Results
RELB transcription and expression were increased in the hippocampus and cortex of epileptic rats during the acute and latent phases and in epileptic foci of patients with temporal lobe epilepsy. Additionally, RelB levels were mainly increased in epileptic rat neurons and accumulated in the nuclei of hippocampal neurons. Further research demonstrated increased GSK3β phosphorylation at the Ser9 inhibitory site and decreased IκBα levels, which contributed to RelB accumulation in hippocampal neurons after seizure and in liposaccharide-stimulated HT22 cells.
Conclusions
This study is the first to demonstrate that RelB is widely distributed and increased in epileptogenic foci neurons in epileptic phenotypes. These results indicate that RelB may play roles in DRE and is mediated by GSK3β and IκBα, providing a new target for anti-epileptic and disease-modifying therapy.
背景:耐药癫痫(DRE)影响着全世界2000多万人。DRE患者对抗癫痫药物无反应。从抗癫痫转向抗癫痫和疾病改善治疗将是未来研究的重要目标。典型核因子κB (NF-κB)信号通路在癫痫和神经炎症中起关键作用。然而,可通过典型和非典型NF-κB信号激活的RelB在癫痫中的表达和调控尚不清楚。为了阐明RelB在DRE表型中的表达和定位,确定RelB调控的相关蛋白,我们进行了以下研究。方法采用定量PCR检测匹罗卡品致痫大鼠RELB的转录水平。Western blotting检测癫痫模型大鼠、DRE患者脑组织及脂多糖诱导的HT22细胞中RelB及RelB调控相关蛋白的丰度。采用免疫荧光染色和免疫组织化学方法对DRE患者脑切片进行RelB定位。ELISA法检测HT22细胞向培养基中分泌的炎性细胞因子。结果癫痫大鼠海马和皮质在急性期和潜伏期以及颞叶癫痫患者的癫痫灶中,relb的转录和表达均有所增加。此外,RelB水平主要在癫痫大鼠神经元中升高,并在海马神经元核中积累。进一步的研究表明,Ser9抑制位点的GSK3β磷酸化增加,i - κ b α水平降低,这有助于癫痫发作后海马神经元和脂多糖刺激的HT22细胞中RelB的积累。结论本研究首次证实了RelB在癫痫表型的致痫灶神经元中广泛分布和增加。这些结果表明,RelB可能在DRE中发挥作用,并通过GSK3β和i- κ b α介导,为抗癫痫和改善疾病治疗提供了新的靶点。