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小鼠少突胶质细胞中的 microRNA 表达及调控蛋白脂质蛋白基因表达。

MicroRNA expression in mouse oligodendrocytes and regulation of proteolipid protein gene expression.

机构信息

Department of Neurology, University of Kentucky, Lexington, Kentucky, USA.

出版信息

J Neurosci Res. 2012 Sep;90(9):1701-12. doi: 10.1002/jnr.23055. Epub 2012 Apr 14.

Abstract

Overexpression of the major myelin proteolipid protein (PLP) is detrimental to brain development and function and is the most common cause of Pelizaeus-Merzbacher disease. microRNA (miRNA), small, noncoding RNAs, have been shown to play critical roles in oligodendrocyte lineage. In this study, we sought to investigate whether miRNAs control PLP abundance. To identify candidate miRNAs involved in this regulation, we have examined differentiation-induced changes in the expression of miRNAs in the oligodendroglial cell line Oli-neu and in enhanced green fluorescent protein positive oligodendrocytes ex vivo. We have identified 145 miRNAs that are expressed in oligodendrocyte cell lineage progression. Dicer1 expression decreases in differentiated oligodendrocytes, and knock down of Dicer1 results in changes in miRNAs similar to those associated with differentiation. To identify miRNAs that control the PLP expression, we have selected miRNAs whose expression is lower in differentiated vs. undifferentiated Oli-neu cells and that have one or more binding site(s) in the PLP 3'-untranslated region (3'UTR). The PLP 3'UTR fused to the luciferase gene reduces the activity of the reporter, suggesting that it negatively regulates message stability or translation. Such suppression is relieved by knock down of miR-20a. Overexpression of miR-20a decreases expression of the endogenous PLP in primary oligodendrocytes and of the reporter gene. Deletion or mutation of the putative binding site for miR-20a in the PLP 3'UTR abrogated such effects. Our data indicate that miRNA expression is regulated by Dicer1 levels in differentiated oligodendrocytes and that miR-20a, a component of the cluster that controls oligodendrocyte cell number, regulates PLP gene expression through its 3'UTR.

摘要

髓鞘主要蛋白脂蛋白(PLP)的过度表达对大脑的发育和功能有害,是佩利兹梅尔巴赫尔病(Pelizaeus-Merzbacher disease)最常见的病因。微小 RNA(miRNA)是一种小的非编码 RNA,在少突胶质细胞谱系中发挥着关键作用。在这项研究中,我们试图研究 miRNA 是否控制 PLP 的丰度。为了鉴定参与这种调控的候选 miRNA,我们检查了少突胶质细胞系 Oli-neu 和体外增强型绿色荧光蛋白阳性少突胶质细胞分化诱导的 miRNA 表达变化。我们鉴定了 145 个在少突胶质细胞谱系进展中表达的 miRNA。Dicer1 在分化的少突胶质细胞中的表达减少,Dicer1 的敲低导致 miRNA 的变化与分化相关的变化相似。为了鉴定控制 PLP 表达的 miRNA,我们选择了在分化的 Oli-neu 细胞中表达水平低于未分化细胞的 miRNA,并且在 PLP 3'非翻译区(3'UTR)中有一个或多个结合位点。PLP 3'UTR 与荧光素酶基因融合降低了报告基因的活性,表明其负调控 mRNA 稳定性或翻译。这种抑制作用通过 miR-20a 的敲低而得到缓解。miR-20a 的过表达降低了原代少突胶质细胞中内源性 PLP 和报告基因的表达。PLP 3'UTR 中 miR-20a 的假定结合位点的缺失或突变消除了这种作用。我们的数据表明,miRNA 的表达受分化的少突胶质细胞中 Dicer1 水平的调节,miR-20a 是控制少突胶质细胞数量的簇的一部分,通过其 3'UTR 调节 PLP 基因的表达。

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