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一种β-肌动蛋白信使核糖核蛋白复合体与邮政编码结合蛋白的定位调节树突丝状伪足和丝状伪足突触的密度。

Localization of a beta-actin messenger ribonucleoprotein complex with zipcode-binding protein modulates the density of dendritic filopodia and filopodial synapses.

作者信息

Eom Taesun, Antar Laura N, Singer Robert H, Bassell Gary J

机构信息

Department of Neuroscience, Rose F. Kennedy Center for Mental Retardation, Albert Einstein College of Medicine, Bronx, New York 10461, USA.

出版信息

J Neurosci. 2003 Nov 12;23(32):10433-44. doi: 10.1523/JNEUROSCI.23-32-10433.2003.

Abstract

The dendritic transport and local translation of mRNA may be an essential mechanism to regulate synaptic growth and plasticity. We investigated the molecular mechanism and function of beta-actin mRNA localization in dendrites of cultured hippocampal neurons. Previous studies have shown that beta-actin mRNA localization to the leading edge of fibroblasts or the growth cones of developing neurites involved a specific interaction between a zipcode sequence in the 3' untranslated region and the mRNA-binding protein zipcode-binding protein-1 (ZBP1). Here, we show that ZBP1 is required for the localization of beta-actin mRNA to dendrites. Knock-down of ZBP1 using morpholino antisense oligonucleotides reduced dendritic levels of ZBP1 and beta-actin mRNA and impaired growth of dendritic filopodia in response to BDNF treatment. Transfection of an enhanced green fluorescent protein (EGFP)-beta-actin construct, which contained the zipcode, increased the density of dendritic filopodia and filopodial synapses. Transfection of an EGFP construct, also with the zipcode, resulted in recruitment of endogenous ZBP1 and beta-actin mRNA into dendrites and similarly increased the density of dendritic filopodia. However, the beta-actin zipcode did not affect filopodial length or the density of mature spines. These results reveal a novel function for an mRNA localization element and its binding protein in the regulation of dendritic morphology and synaptic growth via dendritic filopodia.

摘要

mRNA的树突运输和局部翻译可能是调节突触生长和可塑性的重要机制。我们研究了培养的海马神经元树突中β-肌动蛋白mRNA定位的分子机制和功能。先前的研究表明,β-肌动蛋白mRNA定位于成纤维细胞的前缘或发育中神经突的生长锥,涉及3'非翻译区中的邮政编码序列与mRNA结合蛋白邮政编码结合蛋白-1(ZBP1)之间的特定相互作用。在这里,我们表明ZBP1是β-肌动蛋白mRNA定位于树突所必需的。使用吗啉代反义寡核苷酸敲低ZBP1可降低树突中ZBP1和β-肌动蛋白mRNA的水平,并损害对BDNF处理的树突状丝状伪足的生长。转染包含邮政编码的增强型绿色荧光蛋白(EGFP)-β-肌动蛋白构建体,可增加树突状丝状伪足和丝状伪足突触的密度。同样转染带有邮政编码的EGFP构建体,可导致内源性ZBP1和β-肌动蛋白mRNA募集到树突中,并同样增加树突状丝状伪足的密度。但是,β-肌动蛋白邮政编码不影响丝状伪足的长度或成熟棘的密度。这些结果揭示了mRNA定位元件及其结合蛋白在通过树突状丝状伪足调节树突形态和突触生长中的新功能。

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