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Postsynaptic decoding of neural activity: eEF2 as a biochemical sensor coupling miniature synaptic transmission to local protein synthesis.

机译:突触后神经活动的解码:eEF2作为一种生物化学传感器,将微型突触传递耦合到局部蛋白质合成。

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摘要

Activity-dependent regulation of dendritic protein synthesis is critical for enduring changes in synaptic function, but how the unique features of distinct activity patterns are decoded by the dendritic translation machinery remains poorly understood. Here, we identify eukaryotic elongation factor-2 (eEF2), which catalyzes ribosomal translocation during protein synthesis, as a biochemical sensor in dendrites that is specifically and locally tuned to the quality of neurotransmission. We show that intrinsic action potential (AP)-mediated network activity in cultured hippocampal neurons maintains eEF2 in a relatively dephosphorylated (active) state, whereas spontaneous neurotransmitter release (i.e., miniature neurotransmission) strongly promotes the phosphorylation (and inactivation) of eEF2. The regulation of eEF2 phosphorylation is responsive to bidirectional changes in miniature neurotransmission and is controlled locally in dendrites. Finally, direct spatially controlled inhibition of eEF2 phosphorylation induces local translational activation, suggesting that eEF2 is a biochemical sensor that couples miniature synaptic events to local translational suppression in neuronal dendrites.
机译:树突状蛋白合成的依赖于活性的调节对于持久的突触功能变化至关重要,但是如何通过树突状翻译机制解码不同活动模式的独特特征仍然知之甚少。在这里,我们确定真核伸长因子2(eEF2),其在蛋白质合成过程中催化核糖体易位,作为树突中的生化传感器,具体地和局部地调节至神经传递的质量。我们显示,在培养的海马神经元中内在作用电位(AP)介导的网络活动将eEF2维持在相对去磷酸化(活性)状态,而自发神经递质释放(即微型神经传递)强烈促进eEF2的磷酸化(和失活)。 eEF2磷酸化的调节响应微型神经传递中的双向变化,并在树突状细胞中局部控制。最后,对eEF2磷酸化的直接空间控制抑制可诱导局部翻译激活,这表明eEF2是一种生化传感器,可将微型突触事件与神经元树突中的局部翻译抑制相结合。

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