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TRPC channels regulate Ca2+-signaling and short-term plasticity of fast glutamatergic synapses

机译:TRPC通道调节快速谷氨酸能突触的Ca2 +信号传导和短期可塑性

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摘要

Transient receptor potential (TRP) proteins form Ca2+-permeable, nonselective cation channels, but their role in neuronal Ca2+ homeostasis is elusive. In the present paper, we show that TRPC channels potently regulate synaptic plasticity by changing the presynaptic Ca2+-homeostasis of hippocampal neurons. Specifically, loss of TRPC1/C4/C5 channels decreases basal-evoked secretion, reduces the pool size of readily releasable vesicles, and accelerates synaptic depression during high-frequency stimulation (HFS). In contrast, primary TRPC5 channel-expressing neurons, identified by a novel TRPC5–τ-green fluorescent protein (τGFP) knockin mouse line, show strong short-term enhancement (STE) of synaptic signaling during HFS, indicating a key role of TRPC5 in short-term plasticity. Lentiviral expression of either TRPC1 or TRPC5 turns classic synaptic depression of wild-type neurons into STE, demonstrating that TRPCs are instrumental in regulating synaptic plasticity. Presynaptic Ca2+ imaging shows that TRPC activity strongly boosts synaptic Ca2+ dynamics, showing that TRPC channels provide an additional presynaptic Ca2+ entry pathway, which efficiently regulates synaptic strength and plasticity.
机译:瞬态受体电位(TRP)蛋白形成Ca 2 + -可渗透的非选择性阳离子通道,但是在神经元Ca 2 + 体内稳态中的作用尚不清楚。在本文中,我们表明TRPC通道通过改变海马神经元的突触前Ca 2 + -稳态来有效地调节突触可塑性。具体来说,TRPC1 / C4 / C5通道的丢失会减少基础诱发的分泌,减少易于释放的囊泡的池大小,并在高频刺激(HFS)期间加速突触抑制。相反,由新型TRPC5-τ-绿色荧光蛋白(τGFP)敲入小鼠系鉴定的主要TRPC5通道表达神经元在HFS期间显示突触信号的强短期增强(STE),表明TRPC5在短期可塑性。 TRPC1或TRPC5的慢病毒表达将野生型神经元的经典突触抑制转变为STE,表明TRPC在调节突触可塑性中发挥了作用。突触前Ca 2 + 成像显示TRPC活性强烈增强了突触Ca 2 + 动力学,表明TRPC通道提供了额外的突触前Ca 2 + 进入通路,有效地调节突触强度和可塑性。

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