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Morphine stimulates CCL2 production by human neurons

机译:吗啡刺激人类神经元产生CCL2

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Background Substances of abuse, such as opiates, have a variety of immunomodulatory properties that may influence both neuroinflammatory and neurodegenerative disease processes. The chemokine CCL2, which plays a pivotal role in the recruitment of inflammatory cells in the nervous system, is one of only a few chemokines produced by neurons. We hypothesized that morphine may alter expression of CCL2 by human neurons. Methods Primary neuronal cell cultures and highly purified astrocyte and microglial cell cultures were prepared from human fetal brain tissue. Cell cultures were treated with morphine, and cells were examined by RNase protection assay for mRNA. Culture supernatants were assayed by ELISA for CCL2 protein. β-funaltrexamine (β-FNA) was used to block μ-opioid receptor (MOR)s. Results Morphine upregulated CCL2 mRNA and protein in neuronal cultures in a concentration- and time-dependent fashion, but had no effect on CCL2 production in astrocyte or microglial cell cultures. Immunocytochemical analysis also demonstrated CCL2 production in morphine-stimulated neuronal cultures. The stimulatory effect of morphine was abrogated by β-FNA, indicating an MOR-mediated mechanism. Conclusion Morphine stimulates CCL2 production by human neurons via a MOR-related mechanism. This finding suggests another mechanism whereby opiates could affect neuroinflammatory responses.
机译:背景技术诸如鸦片之类的滥用物质具有多种免疫调节特性,可能会影响神经发炎和神经退行性疾病的进程。趋化因子CCL2在神经系统炎症细胞的募集中起着关键作用,是神经元产生的少数趋化因子之一。我们假设吗啡可能会改变人类神经元的CCL2表达。方法从人胎脑组织中制备原代神经元细胞培养物以及高度纯化的星形胶质细胞和小胶质细胞培养物。用吗啡处理细胞培养物,并通过RNA酶保护试验检测细胞的mRNA。通过ELISA测定培养上清液中的CCL2蛋白。 β-去氨曲明(β-FNA)用于阻断μ阿片受体(MOR)。结果吗啡以浓度和时间依赖性方式上调神经元培养物中的CCL2 mRNA和蛋白,但对星形胶质细胞或小胶质细胞培养物中CCL2的产生没有影响。免疫细胞化学分析还显示了吗啡刺激的神经元培养物中CCL2的产生。 β-FNA消除了吗啡的刺激作用,表明了MOR介导的机制。结论吗啡通过MOR相关机制刺激人神经元产生CCL2。这一发现表明鸦片制剂可以影响神经炎症反应的另一种机制。

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