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Structure of a human cap-dependent 48S translation pre-initiation complex

机译:依赖人类上限的48S翻译预启动复合体的结构

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摘要

Eukaryotic translation initiation is tightly regulated, requiring a set of conserved initiation factors (eIFs). Translation of a capped mRNA depends on the trimeric eIF4F complex and eIF4B to load the mRNA onto the 43S pre-initiation complex comprising 40S and initiation factors 1, 1A, 2, 3 and 5 as well as initiator-tRNA. Binding of the mRNA is followed by mRNA scanning in the 48S pre-initiation complex, until a start codon is recognised. Here, we use a reconstituted system to prepare human 48S complexes assembled on capped mRNA in the presence of eIF4B and eIF4F. The highly purified h-48S complexes are used for cross-linking/mass spectrometry, revealing the protein interaction network in this complex. We report the electron cryo-microscopy structure of the h-48S complex at 6.3 Å resolution. While the majority of eIF4B and eIF4F appear to be flexible with respect to the ribosome, additional density is detected at the entrance of the 40S mRNA channel which we attribute to the RNA-recognition motif of eIF4B. The eight core subunits of eIF3 are bound at the 40S solvent-exposed side, as well as the subunits eIF3d, eIF3b and eIF3i. elF2 and initiator-tRNA bound to the start codon are present at the 40S intersubunit side. This cryo-EM structure represents a molecular snap-shot revealing the h-48S complex following start codon recognition.
机译:真核翻译起始受到严格调节,需要一系列保守的起始因子(eIF)。封端的mRNA的翻译取决于三聚体eIF4F复合物和eIF4B,以将mRNA加载到包含40S和起始因子1、1A,2、3和5以及引发剂-tRNA的43S预起始复合物中。结合mRNA后,在48S预起始复合物中扫描mRNA,直至识别出起始密码子。在这里,我们使用重构的系统来准备在eIF4B和eIF4F存在的情况下在封闭的mRNA上组装的人48S复合物。高度纯化的h-48S复合物用于交联/质谱,揭示了该复合物中的蛋白质相互作用网络。我们以6.3Å的分辨率报告了h-48S复合物的电子冷冻显微镜结构。虽然大多数eIF4B和eIF4F相对于核糖体似乎是柔性的,但在40S mRNA通道的入口处检测到额外的密度,这归因于eIF4B的RNA识别基序。 eIF3的八个核心亚基与eIF3d,eIF3b和eIF3i的亚基结合在40S溶剂暴露的一侧。结合至起始密码子的eIF2和引发剂-tRNA存在于40S亚单位侧。这种低温电磁结构代表分子快照,揭示了起始密码子识别后的h-48S复合物。

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