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Autaptic cultures of human induced neurons as a versatile platform for studying synaptic function and neuronal morphology

机译:人类诱导神经元的自养文化作为研究突触功能和神经元形态的通用平台

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摘要

Recently developed technology to differentiate induced pluripotent stem cells (iPSCs) into human induced neurons (iNs) provides an exciting opportunity to study the function of human neurons. However, functional characterisations of iNs have been hampered by the reliance on mass culturing protocols which do not allow assessment of synaptic release characteristics and neuronal morphology at the individual cell level with quantitative precision. Here, we have developed for the first time a protocol to generate autaptic cultures of iPSC-derived iNs. We show that our method efficiently generates mature, autaptic iNs with robust spontaneous and action potential-driven synaptic transmission. The synaptic responses are sensitive to modulation by metabotropic receptor agonists as well as potentiation by acute phorbol ester application. Finally, we demonstrate loss of evoked and spontaneous release by Unc13A knockdown. This culture system provides a versatile platform allowing for quantitative and integrative assessment of morphophysiological and molecular parameters underlying human synaptic transmission.
机译:最近开发的将诱导多能干细胞(iPSC)分化为人类诱导神经元(iNs)的技术为研究人类神经元的功能提供了令人兴奋的机会。但是,iNs的功能表征已受到对大众培养方案的依赖的困扰,这无法以定量精度评估单个细胞水平上的突触释放特征和神经元形态。在这里,我们首次开发了一种协议来生成iPSC衍生的iN的自闭培养。我们表明,我们的方法有效地生成具有强大的自发性和动作电位驱动的突触传递的成熟,自闭性iNs。突触反应对代谢型受体激动剂的调节以及急性佛波醇酯的增强作用敏感。最后,我们证明了Unc13A敲低引起的诱发性和自发性释放的丧失。该培养系统提供了一个通用平台,可用于定量和综合评估人类突触传递基础的形态生理学和分子参数。

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