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嗜热栖热菌无先导mRNA起始复合物的结构突出了古菌特征和与真核生物的相似性。

Structures of Saccharolobus solfataricus initiation complexes with leaderless mRNAs highlight archaeal features and eukaryotic proximity.

作者信息

Bourgeois Gabrielle, Coureux Pierre-Damien, Lazennec-Schurdevin Christine, Madru Clément, Gaillard Thomas, Duchateau Magalie, Chamot-Rooke Julia, Bourcier Sophie, Mechulam Yves, Schmitt Emmanuelle

机构信息

Laboratoire de Biologie Structurale de la Cellule (BIOC), CNRS, Ecole polytechnique, Institut Polytechnique de Paris, Palaiseau, 91120, France.

Retroviruses and Structural Biochemistry Team, Molecular Microbiology and Structural Biochemistry, UMR 5086 CNRS-Lyon 1, CNRS, Université de Lyon, Lyon, France.

出版信息

Nat Commun. 2025 Jan 2;16(1):348. doi: 10.1038/s41467-024-55718-5.

Abstract

The archaeal ribosome is of the eukaryotic type. TACK and Asgard superphyla, the closest relatives of eukaryotes, have ribosomes containing eukaryotic ribosomal proteins not found in other archaea, eS25, eS26 and eS30. Here, we investigate the case of Saccharolobus solfataricus, a TACK crenarchaeon, using mainly leaderless mRNAs. We characterize the small ribosomal subunit of S. solfataricus bound to SD-leadered or leaderless mRNAs. Cryo-EM structures show eS25, eS26 and eS30 bound to the small subunit. We identify two ribosomal proteins, aS33 and aS34, and an additional domain of eS6. Leaderless mRNAs are bound to the small subunit with contribution of their 5'-triphosphate group. Archaeal eS26 binds to the mRNA exit channel wrapped around the 3' end of rRNA, as in eukaryotes. Its position is not compatible with an SD:antiSD duplex. Our results suggest a positive role of eS26 in leaderless mRNAs translation and possible evolutionary routes from archaeal to eukaryotic translation.

摘要

古菌核糖体属于真核生物类型。真核生物的近亲泉古菌门(TACK)和阿斯加德超门的核糖体含有在其他古菌中未发现的真核核糖体蛋白,即eS25、eS26和eS30。在此,我们主要使用无领导mRNA来研究嗜热栖热菌(一种泉古菌门的泉古菌)的情况。我们对与含SD序列的有领导或无领导mRNA结合的嗜热栖热菌小核糖体亚基进行了表征。冷冻电镜结构显示eS25、eS26和eS30与小亚基结合。我们鉴定出两种核糖体蛋白,即aS33和aS34,以及eS6的一个额外结构域。无领导mRNA通过其5'-三磷酸基团与小亚基结合。与真核生物一样,古菌的eS26与包裹在rRNA 3'端周围的mRNA出口通道结合。其位置与SD:反SD双链不兼容。我们的结果表明eS26在无领导mRNA翻译中具有积极作用,以及从古菌翻译到真核生物翻译可能的进化途径。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/578e/11698992/a938f84e682c/41467_2024_55718_Fig1_HTML.jpg

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