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核糖体结合的 Upf1 形成不同的 80S 复合物并进行 mRNA 监测。

Ribosome-bound Upf1 forms distinct 80S complexes and conducts mRNA surveillance.

机构信息

Department of Microbiology and Physiological Systems, UMass Chan Medical School, Worcester, Massachusetts 01655, USA.

出版信息

RNA. 2022 Dec;28(12):1621-1642. doi: 10.1261/rna.079416.122. Epub 2022 Oct 3.

Abstract

Upf1, Upf2, and Upf3, the central regulators of nonsense-mediated mRNA decay (NMD), appear to exercise their NMD functions while bound to elongating ribosomes, and evidence for this conclusion is particularly compelling for Upf1. Hence, we used selective profiling of yeast Upf1:ribosome association to define that step in greater detail, understand whether the nature of the mRNA being translated influences Upf1:80S interaction, and elucidate the functions of ribosome-associated Upf1. Our approach has allowed us to clarify the timing and specificity of Upf1 association with translating ribosomes, obtain evidence for a Upf1 mRNA surveillance function that precedes the activation of NMD, identify a unique ribosome state that generates 37-43 nt ribosome footprints whose accumulation is dependent on Upf1's ATPase activity, and demonstrate that a mutated form of Upf1 can interfere with normal translation termination and ribosome release. In addition, our results strongly support the existence of at least two distinct functional Upf1 complexes in the NMD pathway.

摘要

Upf1、Upf2 和 Upf3 是无义介导的 mRNA 降解 (NMD) 的核心调节剂,它们似乎在结合延伸核糖体时行使其 NMD 功能,这一结论的证据尤其令人信服的是 Upf1。因此,我们使用酵母 Upf1:核糖体结合的选择性分析来更详细地定义该步骤,了解正在翻译的 mRNA 的性质是否会影响 Upf1:80S 相互作用,并阐明与核糖体结合的 Upf1 的功能。我们的方法使我们能够澄清 Upf1 与翻译核糖体结合的时间和特异性,获得 NMD 激活之前存在 Upf1 mRNA 监测功能的证据,确定产生 37-43nt 核糖体足迹的独特核糖体状态,其积累依赖于 Upf1 的 ATP 酶活性,并证明突变形式的 Upf1 可以干扰正常的翻译终止和核糖体释放。此外,我们的结果强烈支持 NMD 途径中至少存在两种不同功能的 Upf1 复合物。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f882/9670811/3526e79f071a/1621f01.jpg

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