首页> 外文期刊>Nucleic Acids Research >The eukaryotic initiation factor eIF4H facilitates loop-binding, repetitive RNA unwinding by the eIF4A DEAD-box helicase.
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The eukaryotic initiation factor eIF4H facilitates loop-binding, repetitive RNA unwinding by the eIF4A DEAD-box helicase.

机译:真核起始因子eIF4H通过eIF4A DEAD-box解旋酶促进环结合,重复RNA解链。

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摘要

Eukaryotic translation initiation is a highly regulated process in protein synthesis. The principal translation initiation factor eIF4AI displays helicase activity, unwinding secondary structures in the mRNAs 5'-UTR. Single molecule fluorescence resonance energy transfer (sm-FRET) is applied here to directly observe and quantify the helicase activity of eIF4AI in the presence of the ancillary RNA-binding factor eIF4H. Results show that eIF4H can significantly enhance the helicase activity of eIF4AI by strongly binding both to loop structures within the RNA transcript as well as to eIF4AI. In the presence of ATP, the eIF4AI/eIF4H complex exhibits persistent rapid and repetitive cycles of unwinding and re-annealing. ATP titration assays suggest that this process consumes a single ATP molecule per cycle. In contrast, helicase unwinding activity does not occur in the presence of the non-hydrolysable analog ATP-gammaS. Based on our sm-FRET results, we propose an unwinding mechanism where eIF4AI/eIF4H can bind directly to loop structures to destabilize duplexes. Since eIF4AI is the prototypical example of a DEA(D/H)-box RNA helicase, it is highly likely that this unwinding mechanism is applicable to a myriad of DEAD-box helicases employed in RNA metabolism.
机译:真核翻译起始是蛋白质合成中高度受控的过程。主要翻译起始因子eIF4AI显示解旋酶活性,展开mRNA 5'-UTR中的二级结构。在存在辅助RNA结合因子eIF4H的情况下,此处应用单分子荧光共振能量转移(sm-FRET)直接观察和定量eIF4AI的解旋酶活性。结果表明,eIF4H通过与RNA转录物中的环结构以及eIF4AI牢固结合,可以显着增强eIF4AI的解旋酶活性。在存在ATP的情况下,eIF4AI / eIF4H复合物表现出持续的快速且重复的退绕和重新退火循环。 ATP滴定分析表明,此过程每个循环消耗一个ATP分子。相反,在不可水解的类似物ATP-γS存在下,解旋酶解旋活性不发生。根据我们的sm-FRET结果,我们提出了一种展开机制,其中eIF4AI / eIF4H可以直接与环结构结合,从而使双链体不稳定。由于eIF4AI是DEA(D / H)-box RNA解旋酶的原型实例,因此这种展开机制很可能适用于RNA代谢中使用的多种DEAD-box解旋酶。

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