Calsyntenin-1 expression and function in brain tissue of lithium-pilocarpine rat seizure models.

IF 1.6 4区 医学 Q4 NEUROSCIENCES
Synapse Pub Date : 2024-09-01 DOI:10.1002/syn.22307
Fu Zhou, Rong Hu, Yuzhu Wang, Xiaohui Wu, Xuan Chen, Zhiqin Xi, Kebin Zeng
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引用次数: 0

Abstract

To present the expression of calsyntenin-1 (Clstn1) in the brain and investigate the potential mechanism of Clstn1 in lithium-pilocarpine rat seizure models. Thirty-five male SD adult rats were induced to have seizures by intraperitoneal injection of lithium chloride pilocarpine. Rats exhibiting spontaneous seizures were divided into the epilepsy (EP) group (n = 15), whereas those without seizures were divided into the control group (n = 14). Evaluate the expression of Clstn1 in the temporal lobe of two groups using Western blotting, immunohistochemistry, and immunofluorescence. Additionally, 55 male SD rats were subjected to status epilepticus (SE) using the same induction method. Rats experiencing seizures exceeding Racine's level 4 (n = 48) were randomly divided into three groups: SE, SE + control lentivirus (lentiviral vector expressing green fluorescent protein [LV-GFP]), and SE + Clstn1-targeted RNA interference lentivirus (LV-Clstn1-RNAi). The LV-GFP group served as a control for the lentiviral vector, whereas the LV-Clstn1-RNAi group received a lentivirus designed to silence Clstn1 expression. These lentiviral treatments were administered via hippocampal stereotactic injection 2 days after SE induction. Seven days after SE, Western blot analysis was performed to evaluate the expression of Clstn1 in the hippocampus and temporal lobe. Meanwhile, we observed the latency of spontaneous seizures and the frequency of spontaneous seizures within 8 weeks among the three groups. The expression of Clstn1 in the cortex and hippocampus of the EP group was significantly increased compared to the control group (p < .05). Immunohistochemistry and immunofluorescence showed that Clstn1 was widely distributed in the cerebral cortex and hippocampus of rats, and colocalization analysis revealed that it was mainly co expressed with neurons in the cytoplasm. Compared with the SE group (11.80 ± 2.17 days) and the SE + GFP group (12.40 ± 1.67 days), there was a statistically significant difference (p < .05) in the latency period of spontaneous seizures (15.14 ± 2.41 days) in the SE + Clstn1 + RNAi group rats. Compared with the SE group (4.60 ± 1.67 times) and the SE + GFP group (4.80 ± 2.05 times), the SE + Clstn1 + RNAi group (2.0 ± .89 times) showed a significant reduction in the frequency of spontaneous seizures within 2 weeks of chronic phase in rats (p < .05). Elevated Clstn1 expression in EP group suggests its role in EP onset. Targeting Clstn1 may be a potential therapeutic approach for EP management.

锂-匹罗卡品大鼠癫痫模型脑组织中 Calsyntenin-1 的表达和功能。
介绍钙调蛋白-1(Clstn1)在大脑中的表达,并研究Clstn1在氯化锂-皮洛卡品大鼠癫痫模型中的潜在机制。通过腹腔注射氯化锂皮洛卡品诱导35只雄性SD成年大鼠癫痫发作。表现为自发性癫痫发作的大鼠被分为癫痫(EP)组(n = 15),而没有癫痫发作的大鼠被分为对照组(n = 14)。使用 Western 印迹、免疫组织化学和免疫荧光评估两组大鼠颞叶中 Clstn1 的表达。此外,采用相同的诱导方法对 55 只雄性 SD 大鼠进行癫痫状态(SE)诱导。将癫痫发作超过拉辛4级的大鼠(n = 48)随机分为三组:SE、SE + 对照慢病毒(表达绿色荧光蛋白 [LV-GFP] 的慢病毒载体)和 SE + Clstn1 靶向 RNA 干扰慢病毒(LV-Clstn1-RNAi)。LV-GFP 组是慢病毒载体的对照组,而 LV-Clstn1-RNAi 组则接受了旨在抑制 Clstn1 表达的慢病毒。这些慢病毒治疗是在诱导 SE 2 天后通过海马立体定向注射进行的。SE七天后,我们进行了Western印迹分析,以评估Clstn1在海马和颞叶中的表达。同时,我们观察了三组患者自发癫痫发作的潜伏期和8周内自发癫痫发作的频率。与对照组相比,EP 组大脑皮层和海马中 Clstn1 的表达明显增加(p
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来源期刊
Synapse
Synapse 医学-神经科学
CiteScore
3.80
自引率
0.00%
发文量
38
审稿时长
4-8 weeks
期刊介绍: SYNAPSE publishes articles concerned with all aspects of synaptic structure and function. This includes neurotransmitters, neuropeptides, neuromodulators, receptors, gap junctions, metabolism, plasticity, circuitry, mathematical modeling, ion channels, patch recording, single unit recording, development, behavior, pathology, toxicology, etc.
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