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Microdevice for Evaluating Ion Channel Expression by Axon-Targeted Recording to Cultured Neurons*

机译:通过Axon靶向记录对培养的神经元评估离子通道表达的Microdevice *

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Recording axonal conduction will be a strong tool to continuously evaluate Na channel expression of cultured neurons. However, little is known about the relationship between ion channel expression and axonal conduction velocity. In this study, we aim to develop a method to evaluate the relationship. A microdevice was developed with photo- and soft-lithography. Cortical neurons were cultured, and activity propagating along axons was recorded. After spike sorting, mixed signal from multiple axons were sorted into clusters of individual axons. Axons were treated with non-selective and subtype specific Na channel blockers, and changes in conduction delay were evaluated. TTX and lidocaine increased conduction delay with a different manner, suggesting that the different affinity and binding kinetics can be detected with the device. Moreover, although Nav 1.2 blocker increased the conduction delay and eventually clocked the conduction at around IC50, the other blockers did not. This result suggests that Nav 1.2 is dominant for the conduction along unmyelinated cortical axons. Overall, our device should be a feasible tool for elucidating Na channel properties by axon-targeted recording.
机译:记录轴突传导将是一个强大的工具,以连续评估培养神经元的Na通道表达。然而,关于离子通道表达和轴突传导速度之间的关系很少。在这项研究中,我们的目标是开发一种评估关系的方法。使用光链和软光刻开发了微型微型。培养皮质神经元,记录沿轴突传播的活性。在尖峰分选之后,将来自多个轴突的混合信号分类为单个轴突的簇。用非选择性和亚型特异性Na通道阻断剂处理轴突,并评估导电延迟的变化。 TTX和Lidocaine以不同的方式提高导通延迟,表明可以用设备检测不同的亲和力和结合动力学。此外,虽然NAV 1.2阻滞剂增加了导通延迟并最终在IC50周围的传导时,但另一个阻挡者没有。该结果表明,沿着未贴合的皮质轴突的传导是主导的。总的来说,我们的设备应该是通过Axon目标录制阐明Na通道特性的可行工具。

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