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大鼠金属硫蛋白-1信使核糖核酸的核周定位需要3'-非翻译区的一个11个核苷酸的片段。

An eleven nucleotide section of the 3'-untranslated region is required for perinuclear localization of rat metallothionein-1 mRNA.

作者信息

Nury David, Chabanon Hervé, Levadoux-Martin Marilyne, Hesketh John

机构信息

School of Cell and Molecular Biosciences, Faculty of Medicine, University of Newcastle, Newcastle upon Tyne NE1 7RU, UK.

出版信息

Biochem J. 2005 Apr 15;387(Pt 2):419-28. doi: 10.1042/BJ20040630.

Abstract

Localization of mRNAs provides a novel mechanism for synthesis of proteins close to their site of function. MT1 (metallothionein-1) is a small, metal-binding protein that is largely cytoplasmic but which can be found in the nucleus. The localization of rat MT1 requires the perinuclear localization of its mRNA by a mechanism dependent on the 3'-UTR (3'-untranslated region). The present study investigates the nature of this mRNA localization signal using Chinese-hamster ovary cells transfected with gene constructs in which either MT1 or the globin coding region is linked to different sequences from the MT1 3'-UTR. Deletion, mutagenesis and antisense oligonucleotide approaches indicate that nt 45-76 of the 3'-UTR, in particular nt 66-76, are required for the localization of either MT1 mRNA or chimaeric transcripts in which a beta-globin coding region is linked to sequences from the MT1 3'-UTR. This section of the 3'-UTR contains a CACC repeat. Two mutations that are predicted to alter the secondary structure of this region also impair localization. Our hypothesis is that the perinuclear localization signal in MT1 mRNA is formed by a combination of the CACC repeat and its structural context.

摘要

mRNA 的定位为在其功能位点附近合成蛋白质提供了一种新机制。金属硫蛋白 1(MT1)是一种小的金属结合蛋白,主要存在于细胞质中,但也可在细胞核中发现。大鼠 MT1 的定位需要其 mRNA 通过一种依赖于 3'-非翻译区(3'-UTR)的机制进行核周定位。本研究利用转染了基因构建体的中国仓鼠卵巢细胞来研究这种 mRNA 定位信号的性质,在这些构建体中,MT1 或珠蛋白编码区与来自 MT1 3'-UTR 的不同序列相连。缺失、诱变和反义寡核苷酸方法表明,3'-UTR 的第 45 - 76 位核苷酸,特别是第 66 - 76 位核苷酸,是 MT1 mRNA 或嵌合转录本(其中β-珠蛋白编码区与来自 MT1 3'-UTR 的序列相连)定位所必需的。3'-UTR 的这一部分包含一个 CACC 重复序列。预计会改变该区域二级结构的两个突变也会损害定位。我们的假设是,MT1 mRNA 中的核周定位信号是由 CACC 重复序列及其结构背景共同形成的。

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