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肌动蛋白相关的神经结合蛋白-蛋白磷酸酶1复合物调节海马可塑性。

Actin-associated neurabin-protein phosphatase-1 complex regulates hippocampal plasticity.

作者信息

Hu Xiao Dong, Huang Qing, Roadcap David W, Shenolikar Shirish S, Xia Houhui

机构信息

Neuroscience Center of Excellence, LSU Health Science Center, New Orleans, Louisiana, USA.

出版信息

J Neurochem. 2006 Sep;98(6):1841-51. doi: 10.1111/j.1471-4159.2006.04070.x. Epub 2006 Aug 8.

DOI:10.1111/j.1471-4159.2006.04070.x
PMID:16899074
Abstract

Protein phosphatase-1 (PP1) has been implicated in the control of long-term potentiation (LTP) and depression (LTD) in rat hippocampal CA1 neurons. PP1 catalytic subunits associate with multiple postsynaptic regulatory subunits, but the PP1 complexes that control hippocampal LTP and LTD in the rat hippocampus remain unidentified. The neuron-specific actin-binding protein, neurabin-I, is enriched in dendritic spines, and tethers PP1 to actin-rich postsynaptic density to regulate morphology and maturation of spines. The present studies utilized Sindbis virus-mediated expression of wild-type and mutant neurabin-I polypeptides in organotypic cultures of rat hippocampal slices to investigate their role in synaptic plasticity. While wild-type neurabin-I elicited no change in basal synaptic transmission, it enhanced LTD and inhibited LTP in CA1 pyramidal neurons. By comparison, mutant neurabins, specifically those unable to bind PP1 or F-actin, decreased basal synaptic transmission, attenuated LTD and increased LTP in slice cultures. Biochemical and cell biological analyses suggested that, by mislocalizing synaptic PP1, the mutant neurabins impaired the functions of endogenous neurabin-PP1 complexes and modulated LTP and LTD. Together, these studies provided the first biochemical and physiological evidence that a postsynaptic actin-bound neurabin-I-PP1 complex regulates synaptic transmission and bidirectional changes in hippocampal plasticity.

摘要

蛋白磷酸酶-1(PP1)与大鼠海马CA1神经元的长时程增强(LTP)和长时程抑制(LTD)的调控有关。PP1催化亚基与多个突触后调节亚基相关联,但在大鼠海马中控制海马LTP和LTD的PP1复合物仍未明确。神经元特异性肌动蛋白结合蛋白神经肌动蛋白-I在树突棘中富集,并将PP1与富含肌动蛋白的突触后致密物相连,以调节棘的形态和成熟。本研究利用辛德毕斯病毒介导在大鼠海马切片的器官型培养物中表达野生型和突变型神经肌动蛋白-I多肽,以研究它们在突触可塑性中的作用。虽然野生型神经肌动蛋白-I对基础突触传递没有影响,但它增强了LTD并抑制了CA1锥体神经元中的LTP。相比之下,突变型神经肌动蛋白,特别是那些无法结合PP1或F-肌动蛋白的突变型,降低了基础突触传递,减弱了LTD并增加了切片培养物中的LTP。生化和细胞生物学分析表明,通过使突触PP1定位错误,突变型神经肌动蛋白损害了内源性神经肌动蛋白-PP1复合物的功能,并调节了LTP和LTD。总之,这些研究提供了首个生化和生理学证据,即突触后肌动蛋白结合的神经肌动蛋白-I-PP1复合物调节突触传递以及海马可塑性的双向变化。

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