Institute of Anatomy and Molecular Neurobiology, Westfälische Wilhelms-University, 48149 Münster, Germany.
Molecular Physiology Group, Leibniz-Institute of Neurobiology, 39118 Magdeburg, Germany.
J Neurosci. 2018 Sep 19;38(38):8277-8294. doi: 10.1523/JNEUROSCI.0511-18.2018. Epub 2018 Aug 13.
Action potential-evoked neurotransmitter release is impaired in knock-out neurons lacking synaptic cell-adhesion molecules α-neurexins (αNrxns), the extracellularly longer variants of the three vertebrate genes. Ca influx through presynaptic high-voltage gated calcium channels like the ubiquitous P/Q-type (Ca2.1) triggers release of fusion-ready vesicles at many boutons. α2δ Auxiliary subunits regulate trafficking and kinetic properties of Ca2.1 pore-forming subunits but it has remained unclear if this involves αNrxns. Using live cell imaging with Ca indicators, we report here that the total presynaptic Ca influx in primary hippocampal neurons of αNrxn triple knock-out mice of both sexes is reduced and involved lower Ca2.1-mediated transients. This defect is accompanied by lower vesicle release, reduced synaptic abundance of Ca2.1 pore-forming subunits, and elevated surface mobility of α2δ-1 on axons. Overexpression of Nrxn1α in αNrxn triple knock-out neurons is sufficient to restore normal presynaptic Ca influx and synaptic vesicle release. Moreover, coexpression of Nrxn1α together with α2δ-1 subunits facilitates Ca influx further but causes little augmentation together with a different subunit, α2δ-3, suggesting remarkable specificity. Expression of defined recombinant Ca2.1 channels in heterologous cells validates and extends the findings from neurons. Whole-cell patch-clamp recordings show that Nrxn1α in combination with α2δ-1, but not with α2δ-3, facilitates Ca currents of recombinant Ca2.1 without altering channel kinetics. These results suggest that presynaptic Nrxn1α acts as a positive regulator of Ca influx through Ca2.1 channels containing α2δ-1 subunits. We propose that this regulation represents an important way for neurons to adjust synaptic strength. Synaptic transmission between neurons depends on the fusion of neurotransmitter-filled vesicles with the presynaptic membrane, which subsequently activates postsynaptic receptors. Influx of calcium ions into the presynaptic terminal is the key step to trigger vesicle release and involves different subtypes of voltage-gated calcium channels. We study the regulation of calcium channels by neurexins, a family of synaptic cell-adhesion molecules that are essential for many synapse properties. Using optical measurements of calcium influx in cultured neurons and electrophysiological recordings of calcium currents from recombinant channels, we show that a major neurexin variant facilitates calcium influx through P/Q-type channels by interacting with their α2δ-1 auxiliary subunits. These results propose a novel way how neurons can modulate the strength of distinct synapses.
动作电位诱发的神经递质释放受损,在缺乏突触细胞粘附分子α-neurexins(αNrxns)的敲除神经元中,αNrxns 是三种脊椎动物基因中细胞外较长的变体。通过像普遍存在的 P/Q 型(Ca2.1)这样的突触前高电压门控钙通道的 Ca 流入,触发许多囊泡的融合准备释放。α2δ辅助亚基调节 Ca2.1 孔形成亚基的运输和动力学特性,但尚不清楚这是否涉及到αNrxns。使用带有 Ca 指示剂的活细胞成像,我们在此报告,两性原发性海马神经元中 αNrxn 三重敲除小鼠的总突触前 Ca 流入减少,涉及较低的 Ca2.1 介导的瞬变。这种缺陷伴随着较低的囊泡释放、Ca2.1 孔形成亚基的突触丰度降低和轴突上α2δ-1 的表面迁移率升高。在 αNrxn 三重敲除神经元中过表达 Nrxn1α 足以恢复正常的突触前 Ca 流入和突触囊泡释放。此外,Nrxn1α 与α2δ-1 亚基的共表达进一步促进 Ca 流入,但与不同的亚基α2δ-3 一起引起的扩增很小,表明存在显著的特异性。在异源细胞中表达定义的重组 Ca2.1 通道验证并扩展了神经元中的发现。全细胞膜片钳记录显示,Nrxn1α 与α2δ-1 结合,但与α2δ-3 结合,可促进重组 Ca2.1 电流而不改变通道动力学。这些结果表明,突触前 Nrxn1α 作为通过包含α2δ-1 亚基的 Ca2.1 通道的 Ca 流入的正调节剂发挥作用。我们提出,这种调节代表了神经元调整突触强度的重要方式。神经元之间的突触传递依赖于充满神经递质的囊泡与突触前膜的融合,随后激活突触后受体。Ca2+ 离子流入突触前末梢是触发囊泡释放的关键步骤,涉及不同类型的电压门控钙通道。我们研究了神经递质对钙通道的调节作用,神经递质是一种突触细胞粘附分子家族,对许多突触特性都是必不可少的。使用培养神经元中钙流入的光学测量和重组通道中钙电流的电生理记录,我们表明,一种主要的神经递质变体通过与 P/Q 型通道的α2δ-1 辅助亚基相互作用促进 Ca2+ 流入。这些结果提出了一种新的方式,神经元可以调节不同突触的强度。
