大麻素对 SH-SY5Y 细胞培养模型中突触标记的影响。

IF 3 Q2 PSYCHIATRY Schizophrenia (Heidelberg, Germany) Pub Date : 2024-10-25 DOI:10.1038/s41537-024-00498-6
Kirsten Jahn, Nina Blumer, Caroline Wieltsch, Laura Duzzi, Heiko Fuchs, Roland Meister, Adrian Groh, Martin Schulze Westhoff, Tillmann Horst Christoph Krüger, Stefan Bleich, Abdul Qayyum Khan, Helge Frieling
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引用次数: 0

摘要

与健康人相比,精神分裂症患者的突触连通性会降低,而且通常在精神分裂症发病前就会吸食大麻。因此,我们在 SH-SY5Y 细胞培养模型中研究了不同类型的大麻素是否会影响与突触的发育和保存以及突触功能有关的精神分裂症候选基因的甲基化模式和表达。为此,SH-SY5Y 细胞被分化成神经元样细胞类型,如前所述。通过分析细胞形态、测量神经元/树突长度以及确定与突触形成有关的不同靶分子的甲基化模式、表达(实时 qPCR、Western 印迹)和定位(免疫细胞化学),研究了大麻素 delta-9-THC、HU-210 和 Anandamide 的作用。就形态学的总体印象而言,与单独使用维甲酸(RA)相比,在使用三种大麻素的情况下,细胞和神经元似乎更加扁平/圆润,有更多的结构可以大胆地描述为类似于运输泡。不过,三种大麻素之间并无明显差异。在树突或树枝长度方面,RA 处理细胞的树突和树枝长度明显长于未分化对照细胞(如前所述),但大麻素处理与单独施用 RA 之间没有差异。经大麻素处理的细胞中突触候选基因启动子区域的甲基化率介于分化细胞和未处理对照组之间,尽管仅在部分调查基因中发现了显著差异。除结构分子(NEFH、MAPT)外,大多数调查靶标的 mRNA 水平也显示出同样的趋势,即在应用三种大麻素后,其值接近未分化对照组。同样,通过 Western 印迹分析对表达进行量化后发现,与未分化对照组相比,经 RA 处理的细胞中靶标的表达量更高,而在额外应用 THC 的情况下,靶标的表达量呈下降趋势。与我们之前的研究结果一致,应用 RA 会导致 ICC 中大多数研究靶标的荧光强度升高和/或在细胞中出现不同的信号分布。在使用 THC 的情况下,荧光强度下降,或信号分布变得与未分化对照条件下的分布相似。我们的研究结果表明,在应用大麻素的情况下,我们的体外细胞培养系统中的神经元分化标志物会下降。
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Impact of cannabinoids on synapse markers in an SH-SY5Y cell culture model.

Patients suffering from schizophrenic psychosis show reduced synaptic connectivity compared to healthy individuals, and often, the use of cannabis precedes the onset of schizophrenic psychosis. Therefore, we investigated if different types of cannabinoids impact methylation patterns and expression of schizophrenia candidate genes concerned with the development and preservation of synapses and synaptic function in a SH-SY5Y cell culture model. For this purpose, SH-SY5Y cells were differentiated into a neuron-like cell type as previously described. Effects of the cannabinoids delta-9-THC, HU-210, and Anandamide were investigated by analysis of cell morphology and measurement of neurite/dendrite lengths as well as determination of methylation pattern, expression (real time-qPCR, western blot) and localization (immunocytochemistry) of different target molecules concerned with the formation of synapses. Regarding the global impression of morphology, cells, and neurites appeared to be a bit more blunted/roundish and to have more structures that could be described a bit boldly as resembling transport vesicles under the application of the three cannabinoids in comparison to a sole application of retinoic acid (RA). However, there were no obvious differences between the three cannabinoids. Concerning dendrites or branch lengths, there was a significant difference with longer dendrites and branches in RA-treated cells than in undifferentiated control cells (as shown previously), but there were no differences between cannabinoid treatment and exclusive RA application. Methylation rates in the promoter regions of synapse candidate genes in cannabinoid-treated cells were in between those of differentiated cells and untreated controls, even though findings were significant only in some of the investigated genes. In other targets, the methylation rates of cannabinoid-treated cells did not only approach those of undifferentiated cells but were also valued even beyond. mRNA levels also showed the same tendency of values approaching those of undifferentiated controls under the application of the three cannabinoids for most investigated targets except for the structural molecules (NEFH, MAPT). Likewise, the quantification of expression via western blot analysis revealed a higher expression of targets in RA-treated cells compared to undifferentiated controls and, again, lower expression under the additional application of THC in trend. In line with our earlier findings, the application of RA led to higher fluorescence intensity and/or a differential signal distribution in the cell in most of the investigated targets in ICC. Under treatment with THC, fluorescence intensity decreased, or the signal distribution became similar to the dispersion in the undifferentiated control condition. Our findings point to a decline of neuronal differentiation markers in our in vitro cell-culture system under the application of cannabinoids.

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