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Staufen 2 调控海马神经元中 mGluR 的长时程抑制和 Map1b mRNA 的分布。

Staufen 2 regulates mGluR long-term depression and Map1b mRNA distribution in hippocampal neurons.

机构信息

Département de physiologie, GRSNC, Université de Montréal, Montréal, Québec H3C 3J7, Canada.

出版信息

Learn Mem. 2011 Apr 20;18(5):314-26. doi: 10.1101/lm.2100611. Print 2011.

DOI:10.1101/lm.2100611
PMID:21508097
Abstract

The two members of the Staufen family of RNA-binding proteins, Stau1 and Stau2, are present in distinct ribonucleoprotein complexes and associate with different mRNAs. Stau1 is required for protein synthesis-dependent long-term potentiation (L-LTP) in hippocampal pyramidal cells. However, the role of Stau2 in synaptic plasticity remains unexplored. We found that unlike Stau1, Stau2 is not required for L-LTP. In contrast, Stau2, but not Stau1, is necessary for DHPG-induced protein synthesis-dependent long-term depression (mGluR-LTD). While Stau2 is involved in early development of spines, its down-regulation does not alter spine morphology or spontaneous miniature synaptic activity in older cultures where LTD occurs. In addition, Stau2, but not Stau1, knockdown reduces the dendritic localization of Map1b mRNA, a specific transcript involved in mGluR-LTD. Moreover, mGluR stimulation with DHPG induces Map1b, but not Map2, mRNA dissociation from mRNA granules containing Stau2 and the ribosomal protein P0. This dissociation was not observed in cells in which Stau2 was depleted. Finally, Stau2 knockdown reduces basal Map1b protein expression in dendrites and prevents DHPG-induced increases in dendritic Map1b protein level. We suggest a role for Stau2 in the generation and regulation of Map1b mRNA containing granules that are required for mGluR-LTD.

摘要

Staufen 家族的两个 RNA 结合蛋白成员 Stau1 和 Stau2 存在于不同的核糖核蛋白复合物中,并与不同的 mRNA 结合。Stau1 是海马锥体神经元中依赖蛋白合成的长时程增强(L-LTP)所必需的。然而,Stau2 在突触可塑性中的作用仍未被探索。我们发现,与 Stau1 不同,Stau2 不是 L-LTP 所必需的。相反,Stau2 而不是 Stau1 是 DHPG 诱导的依赖蛋白合成的长时程抑制(mGluR-LTD)所必需的。虽然 Stau2 参与了棘突的早期发育,但在发生 LTD 的较老培养物中,其下调不会改变棘突形态或自发微小突触活性。此外,Stau2 而不是 Stau1 的敲低减少了 Map1b mRNA 的树突定位,Map1b mRNA 是一种参与 mGluR-LTD 的特定转录本。此外,用 DHPG 刺激 mGluR 会诱导 Map1b mRNA 从含有 Stau2 和核糖体蛋白 P0 的 mRNA 颗粒中解离,但在耗尽 Stau2 的细胞中未观察到这种解离。最后,Stau2 敲低减少了树突中 Map1b 蛋白的基础表达,并阻止了 DHPG 诱导的树突 Map1b 蛋白水平的增加。我们提出了 Stau2 在生成和调节含有 Map1b mRNA 的颗粒中的作用,这些颗粒对于 mGluR-LTD 是必需的。

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