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Botulinum Toxin Suppression of CNS Network Activity In Vitro

机译:肉毒毒素体外抑制中枢神经系统网络活动

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摘要

The botulinum toxins are potent agents which disrupt synaptic transmission. While the standard method for BoNT detection and quantification is based on the mouse lethality assay, we have examined whether alterations in cultured neuronal network activity can be used to detect the functional effects of BoNT. Murine spinal cord and frontal cortex networks cultured on substrate integrated microelectrode arrays allowed monitoring of spontaneous spike and burst activity with exposure to BoNT serotype A (BoNT-A). Exposure to BoNT-A inhibited spike activity in cultured neuronal networks where, after a delay due to toxin internalization, the rate of activity loss depended on toxin concentration. Over a 30 hr exposure to BoNT-A, the minimum concentration detected was 2 ng/mL, a level consistent with mouse lethality studies. A small proportion of spinal cord networks, but not frontal cortex networks, showed a transient increase in spike and burst activity with exposure to BoNT-A, an effect likely due to preferential inhibition of inhibitory synapses expressed in this tissue. Lastly, prior exposure to human-derived antisera containing neutralizing antibodies prevented BoNT-A induced inhibition of network spike activity. These observations suggest that the extracellular recording from cultured neuronal networks can be used to detect and quantify functional BoNT effects.
机译:肉毒杆菌毒素是破坏突触传递的有效剂。虽然用于BoNT检测和定量的标准方法是基于小鼠杀伤力测定,但我们已经检查了培养的神经元网络活动的改变是否可用于检测BoNT的功能作用。在整合了基质的微电极阵列上培养的小鼠脊髓和额叶皮层网络可监测暴露于BoNT血清型A(BoNT-A)的自发性突增和爆发活动。暴露于BoNT-A会抑制培养的神经元网络中的突波活性,在此过程中,由于毒素内在化而延迟后,活性丧失的速度取决于毒素浓度。在BoNT-A暴露30小时后,检测到的最低浓度为2µng / mL,该水平与小鼠致死性研究一致。一小部分的脊髓网络(而不是额叶皮层网络)在暴露于BoNT-A时显示出突波和猝发活动的短暂增加,这可能是由于优先抑制在该组织中表达的抑制性突触所致。最后,事先暴露于人源的含中和抗体的抗血清可防止BoNT-A诱导的网络刺突活性抑制。这些观察结果表明,来自培养的神经元网络的细胞外记录可用于检测和量化功能性BoNT效应。

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