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Inorganic polyphosphate regulates neuronal excitability through modulation of voltage-gated channels

机译:无机多磷酸盐通过调制电压门控通道来调节神经元兴奋性

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Background Inorganic polyphosphate (polyP) is a highly charged polyanion capable of interacting with a number of molecular targets. This signaling molecule is released into the extracellular matrix by central astrocytes and by peripheral platelets during inflammation. While the release of polyP is associated with both induction of blood coagulation and astrocyte extracellular signaling, the role of secreted polyP in regulation of neuronal activity remains undefined. Here we test the hypothesis that polyP is an important participant in neuronal signaling. Specifically, we investigate the ability of neurons to release polyP and to induce neuronal firing, and clarify the underlying molecular mechanisms of this process by studying the action of polyP on voltage gated channels. Results Using patch clamp techniques, and primary hippocampal and dorsal root ganglion cell cultures, we demonstrate that polyP directly influences neuronal activity, inducing action potential generation in both PNS and CNS neurons. Mechanistically, this is accomplished by shifting the voltage sensitivity of NaV channel activation toward the neuronal resting membrane potential, the block KV channels, and the activation of CaV channels. Next, using calcium imaging we found that polyP stimulates an increase in neuronal network activity and induces calcium influx in glial cells. Using in situ DAPI localization and live imaging, we demonstrate that polyP is naturally present in synaptic regions and is released from the neurons upon depolarization. Finally, using a biochemical assay we demonstrate that polyP is present in synaptosomes and can be released upon their membrane depolarization by the addition of potassium chloride. Conclusions We conclude that polyP release leads to increased excitability of the neuronal membrane through the modulation of voltage gated ion channels. Together, our data establishes that polyP could function as excitatory neuromodulator in both the PNS and CNS.
机译:背景技术无机多磷酸盐(息肉)是能够与许多分子靶标相互作用的高电荷的聚膜。该信号分子通过中央星形胶质细胞和炎症期间的外周血小板释放到细胞外基质中。虽然息肉释放与血液凝血和星形胶质细胞细胞外信号传导的诱导相关,但分泌息肉在神经元活动调节中的作用仍未确定。在这里,我们测试息肉是神经元信令的重要参与者的假设。具体而言,我们研究神经元释放息肉并诱导神经元烧制的能力,并通过研究息肉对电压门控通道的作用来阐明该过​​程的底层分子机制。结果采用膜片钳技术和原发性海马和背根神经节细胞培养物,我们证明息肉直接影响神经元活动,诱导PNS和CNS神经元中的动作电位产生。机械地,这是通过将NAV通道激活朝向神经元静态膜电位,块KV通道和CaV通道的激活来实现的实现来实现的。接下来,使用钙成像我们发现息肉刺激神经元网络活性的增加,并在胶质细胞中诱导钙流入。使用原位DAPI本地化和实时成像,我们证明息肉在突触区域中自然存在,并且在去极化时从神经元释放。最后,使用生物化学测定,我们证明了突出蛋白酶中存在息肉,并且可以通过加入氯化钾在它们的膜去极化上释放。结论我们得出结论,息肉释放导致通过电压门控离子通道的调制增加神经元膜的兴奋性。我们的数据在一起建立了息肉可以在PNS和CNS中用作兴奋性神经调节器。

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