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荧光标记的人 eIF3 用于单分子光谱学。

Fluorescently-tagged human eIF3 for single-molecule spectroscopy.

机构信息

Department of Chemical and Systems Biology, Stanford University, Stanford, CA 94305, USA.

Department of Structural Biology, Stanford University, Stanford, CA 94305, USA.

出版信息

Nucleic Acids Res. 2018 Jan 25;46(2):e8. doi: 10.1093/nar/gkx1050.

Abstract

Human translation initiation relies on the combined activities of numerous ribosome-associated eukaryotic initiation factors (eIFs). The largest factor, eIF3, is an ∼800 kDa multiprotein complex that orchestrates a network of interactions with the small 40S ribosomal subunit, other eIFs, and mRNA, while participating in nearly every step of initiation. How these interactions take place during the time course of translation initiation remains unclear. Here, we describe a method for the expression and affinity purification of a fluorescently-tagged eIF3 from human cells. The tagged eIF3 dodecamer is structurally intact, functions in cell-based assays, and interacts with the HCV IRES mRNA and the 40S-IRES complex in vitro. By tracking the binding of single eIF3 molecules to the HCV IRES RNA with a zero-mode waveguides-based instrument, we show that eIF3 samples both wild-type IRES and an IRES that lacks the eIF3-binding region, and that the high-affinity eIF3-IRES interaction is largely determined by slow dissociation kinetics. The application of single-molecule methods to more complex systems involving eIF3 may unveil dynamics underlying mRNA selection and ribosome loading during human translation initiation.

摘要

人类翻译起始依赖于众多核糖体相关的真核起始因子(eIFs)的共同活动。最大的因子 eIF3 是一个约 800 kDa 的多蛋白复合物,它与小的 40S 核糖体亚基、其他 eIFs 和 mRNA 协调相互作用网络,同时参与起始的几乎每一个步骤。这些相互作用在翻译起始的时间过程中是如何发生的仍然不清楚。在这里,我们描述了一种从人细胞中表达和亲和纯化荧光标记的 eIF3 的方法。标记的 eIF3 十二聚体结构完整,在基于细胞的测定中起作用,并在体外与 HCV IRES mRNA 和 40S-IRES 复合物相互作用。通过使用基于零模式波导的仪器跟踪单个 eIF3 分子与 HCV IRES RNA 的结合,我们表明 eIF3 既可以与野生型 IRES 结合,也可以与缺乏 eIF3 结合区的 IRES 结合,并且高亲和力的 eIF3-IRES 相互作用主要由缓慢的解离动力学决定。将单分子方法应用于更复杂的涉及 eIF3 的系统,可能会揭示人类翻译起始过程中 mRNA 选择和核糖体加载的动力学。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8ba0/5778468/978d7722b494/gkx1050fig1.jpg

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