首页> 美国卫生研究院文献>Molecular and Cellular Biology >Vertebrate mRNAs with a 5-terminal pyrimidine tract are candidates for translational repression in quiescent cells: characterization of the translational cis-regulatory element.
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Vertebrate mRNAs with a 5-terminal pyrimidine tract are candidates for translational repression in quiescent cells: characterization of the translational cis-regulatory element.

机译:具有5末端嘧啶段的脊椎动物mRNA是静止细胞中翻译抑制的候选者:翻译顺式调节元件的表征。

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摘要

The translation of mammalian ribosomal protein (rp) mRNAs is selectively repressed in nongrowing cells. This response is mediated through a regulatory element residing in the 5' untranslated region of these mRNAs and includes a 5' terminal oligopyrimidine tract (5' TOP). To further characterize the translational cis-regulatory element, we monitored the translational behavior of various endogenous and heterologous mRNAs or hybrid transcripts derived from transfected chimeric genes. The translational efficiency of these mRNAs was assessed in cells that either were growing normally or were growth arrested under various physiological conditions. Our experiments have yielded the following results: (i) the translation of mammalian rp mRNAs is properly regulated in amphibian cells, and likewise, amphibian rp mRNA is regulated in mammalian cells, indicating that all of the elements required for translation control of rp mRNAs are conserved among vertebrate classes; (ii) selective translational control is not confined to rp mRNAs, as mRNAs encoding the naturally occurring ubiquitin-rp fusion protein and elongation factor 1 alpha, which contain a 5' TOP, also conform this mode of regulation; (iii) rat rpP2 mRNA contains only five pyrimidines in its 5' TOP, yet this mRNA is translationally controlled in the same fashion as other rp mRNAs with a 5' TOP of eight or more pyrimidines; (iv) full manifestation of this mode of regulation seems to require both the 5' TOP and sequences immediately downstream; and (v) an intact translational regulatory element from rpL32 mRNA fails to exert its regulatory properties even when preceded by a single A residue.
机译:哺乳动物核糖体蛋白(rp)mRNA的翻译在非生长细胞中被选择性抑制。该反应通过位于这些mRNA的5'非翻译区的调控元件介导,包括5'末端寡嘧啶片段(5'TOP)。为了进一步表征翻译顺式调控元件,我们监测了各种内源性和异源性mRNA或衍生自转染嵌合基因的杂种转录本的翻译行为。在正常生长或在各种生理条件下被阻止生长的细胞中评估了这些mRNA的翻译效率。我们的实验得出以下结果:(i)在两栖动物细胞中哺乳动物rp mRNA的翻译受到适当调节,同样,在哺乳动物细胞中两栖动物rp mRNA也受到调节​​,这表明rp mRNA的翻译控制所需的所有元素都是在脊椎动物中是保守的; (ii)选择性翻译控制不限于rp mRNA,因为编码天然存在的泛素-rp融合蛋白和包含5'TOP的延伸因子1 alpha的mRNA也符合这种调节方式; (iii)大鼠rpP2 mRNA在其5'TOP中仅含有5个嘧啶,但该mRNA的翻译控制方式与其他具有8个或更多嘧啶的5'TOP的rp mRNA相同。 (iv)这种调节方式的充分表现似乎需要5'TOP和紧接下游的序列; (v)来自rpL32 mRNA的完整翻译调控元件即使在前面带有单个A残基的情况下也无法发挥其调控特性。

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