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Characterization of rat spinal cord neurons cultured in defined media on microelectrode arrays.

机译:在微电极阵列上定义的培养基中培养的大鼠脊髓神经元的表征。

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Previous efforts to utilize mammalian spinal cord neurons as biosensor elements have relied on neuronal: glial co-cultures maintained in serum-containing media. We have examined the feasibility of culturing primary spinal cord neurons in serum-free medium, modified for neuronal longevity, on fabricated microelectrode arrays. Embryonic day 15 rat spinal cord cells were plated on trimethoxysilyl-propyldiethylenetriamine coated microelectrode arrays comprised of gold recording sites passivated with silicon nitride. Immunocytochemistry was performed to verify the presence of neurons and quantitatively assess astrocytes using antibodies against glial fibrillary acidic protein on the silicon nitride substrates. Modifications to culture media enabled viable neuronal culture to extend from approximately 14 days in vitro (DIV) to 40 DIV on the arrays containing only 1.1 +/- 0.5% (mean +/- SEM) astrocytes. Extracellular recording revealed tetrodotoxin-sensitive spontaneous electrical activity from the enriched neuronal culture. Threshold detection of extracellular potentials showed an increase in spike rate as a function of glutamate concentration with neurotoxicity at elevated levels. This approach suggests that functional measures related to biosensor applications, pharmacological screening, or the evaluation of neurological disease models can be implemented in a defined culture system.
机译:利用哺乳动物脊髓神经元作为生物传感器元件的先前努力依赖于神经元:在含血清的培养基中维持的神经胶质共培养。我们已经检查了在微电极阵列上在无血清培养基中培养原代脊髓神经元的可行性,该培养基针对神经元寿命进行了改良。将胚胎第15天的大鼠脊髓细胞铺在三甲氧基甲硅烷基-丙基二亚乙基三胺涂覆的微电极阵列上,该微电极阵列由用氮化硅钝化的金记录位点组成。进行了免疫细胞化学检查,以验证神经元的存在并使用氮化硅底物上的神经胶质纤维酸性蛋白的抗体定量评估星形胶质细胞。对培养基的修饰使得在仅包含1.1 +/- 0.5%(平均+/- SEM)星形胶质细胞的阵列上,可行的神经元培养能够从体外大约14天(DIV)扩展到40 DIV。细胞外记录显示丰富的神经元培养物中河豚毒素敏感的自发电活动。胞外电位的阈值检测显示,随着谷氨酸浓度的升高,尖峰频率增加,神经毒性水平升高。这种方法表明,可以在定义的培养系统中实施与生物传感器应用,药理筛选或神经疾病模型评估相关的功能性措施。

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