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Real-Time Amperometric Measurements of Zeptomole Quantities of Dopamine Released from Neurons

机译:实时安培法测量神经元释放的多巴胺的分子数量。

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Amperometry with carbon-fiber microelectrodes provides a unique way to measure very small chemical concentration changes at the surface of biological cells. In this work, an investigation of dopamine release from individual neurons isolated from the mouse retina is described. The mice were genetically modified so that, in cells that expressed the protein responsible for catecholamine synthesis, tyrosine hydroxylase, the marker protein, placental alkaline phosphatase, was also expressed. This modification allowed for identification of the dopamine-containing cells among the many present in the freshly dissociated retina. Release of dopamine was evoked by chemical secretagogues delivered from micropipets that were calibrated with respect to response time and concentration delivered. Amperometric measurements were recorded with low-noise patch clamp amplifiers, and the primary noise source was found to be the electrode capacitance. Dopamine release occurred in the form of transient concentration spikes, consistent with release from small intracellular vesicles. With optimized filtering of the data, the quantity secreted during each release event could be determined. The average quantity determined at one cell was 52 zmol. However, the spikes were quite variable in size and the amount released per event ranged from 8 to 170 zmol. These measurements allow an estimation of the concentration of released transmitter in a synapse.
机译:碳纤维微电极的电流分析法提供了一种独特的方法来测量生物细胞表面的很小的化学浓度变化。在这项工作中,描述了从小鼠视网膜分离的单个神经元释放多巴胺的研究。对小鼠进行了基因改造,以便在表达负责儿茶酚胺合成的蛋白的细胞中,酪氨酸羟化酶,标志物蛋白,胎盘碱性磷酸酶也得以表达。这种修饰允许在新鲜分离的视网膜中存在的许多细胞中鉴定出含多巴胺的细胞。多巴胺的释放是由从微量移液管中释放出来的化学促分泌素引起的,这些化学促分泌剂根据响应时间和释放的浓度进行了校准。用低噪声膜片钳放大器记录安培测量值,发现主要噪声源是电极电容。多巴胺的释放以瞬时浓度峰值的形式发生,与小细胞内囊泡的释放一致。通过优化的数据过滤,可以确定每个释放事件期间的分泌量。在一个电池中测定的平均量为52zmol。但是,尖峰的大小变化很大,每次事件释放的量为8至170 zmol。这些测量值可以估算突触中释放的发射器的浓度。

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