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Directed hydroxyl radical probing reveals Upf1 binding to the 80S ribosomal E site rRNA at the L1 stalk

机译:定向羟基自由基探测揭示了Upf1与L1茎上的80S核糖体E位点rRNA结合

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摘要

Upf1 is an SF1-family RNA helicase that is essential for the nonsense-mediated decay (NMD) process in eukaryotes. While Upf1 has been shown to interact with 80S ribosomes, the molecular details of this interaction were unknown. Using purified recombinant proteins and high-throughput sequencing combined with Fe-BABE directed hydroxyl radical probing (HTS-BABE) we have characterized the interaction between Upf1 and the yeast 80S ribosome. We identify the 1C domain of Upf1, an alpha-helical insertion in the RecA helicase core, to be essential for ribosome binding, and determine that the L1 stalk of 25S rRNA is the binding site for Upf1 on the ribosome. Using the cleavage sites identified by hydroxyl radical probing and high-resolution structures of both yeast Upf1 and the human 80S ribosome, we provide a model of a Upf1:80S structure. Our model requires that the L1 stalk adopt an open configuration as adopted by an un-rotated, or classical-state, ribosome. Our results shed light on the interaction between Upf1 and the ribosome, and suggest that Upf1 may specifically engage a classical-state ribosome during translation.
机译:Upf1是一种SF1家族RNA解旋酶,对于真核生物的无意义介导的衰变(NMD)过程至关重要。尽管已证明Upf1与80S核糖体相互作用,但这种相互作用的分子细节尚不清楚。使用纯化的重组蛋白和高通量测序结合Fe-BABE指导的羟基自由基探测(HTS-BABE),我们已经表征了Upf1和酵母80S核糖体之间的相互作用。我们确定Upf1的1C结构域,在RecA解旋酶核心中的α螺旋插入,对于核糖体结合必不可少,并确定25S rRNA的L1茎是Upf1在核糖体上的结合位点。使用通过羟基自由基探测和酵母Upf1和人类80S核糖体的高分辨率结构鉴定的切割位点,我们提供了Upf1:80S结构的模型。我们的模型要求L1茎采用未旋转或经典状态的核糖体所采用的开放构型。我们的研究结果揭示了Upf1与核糖体之间的相互作用,并暗示Upf1在翻译过程中可能特异性地参与了经典状态的核糖体。

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