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一个 Pcc1 的旁系同源物是古菌 KEOPS tRNA 修饰复合物的第五个核心亚基。

A paralog of Pcc1 is the fifth core subunit of the KEOPS tRNA-modifying complex in Archaea.

机构信息

Université Paris-Saclay, CEA, CNRS, Institute for Integrative Biology of the Cell (I2BC), 91198, Gif-sur-Yvette, France.

Department of structural biology and chemistry, Institut Pasteur, Paris, France.

出版信息

Nat Commun. 2023 Feb 1;14(1):526. doi: 10.1038/s41467-023-36210-y.

Abstract

In Archaea and Eukaryotes, the synthesis of a universal tRNA modification, N-threonyl-carbamoyl adenosine (tA), is catalyzed by the KEOPS complex composed of Kae1, Bud32, Cgi121, and Pcc1. A fifth subunit, Gon7, is found only in Fungi and Metazoa. Here, we identify and characterize a fifth KEOPS subunit in Archaea. This protein, dubbed Pcc2, is a paralog of Pcc1 and is widely conserved in Archaea. Pcc1 and Pcc2 form a heterodimer in solution, and show modest sequence conservation but very high structural similarity. The five-subunit archaeal KEOPS does not form dimers but retains robust tRNA binding and tA synthetic activity. Pcc2 can substitute for Pcc1 but the resulting KEOPS complex is inactive, suggesting a distinct function for the two paralogs. Comparative sequence and structure analyses point to a possible evolutionary link between archaeal Pcc2 and eukaryotic Gon7. Our work indicates that Pcc2 regulates the oligomeric state of the KEOPS complex, a feature that seems to be conserved from Archaea to Eukaryotes.

摘要

在古菌和真核生物中,普遍的 tRNA 修饰 N-硫代羰基腺苷(tA)的合成由 KEOPS 复合物催化,该复合物由 Kae1、Bud32、Cgi121 和 Pcc1 组成。第五个亚基 Gon7 仅存在于真菌和后生动物中。在这里,我们在古菌中鉴定并表征了第五个 KEOPS 亚基。这种蛋白质被称为 Pcc2,是 Pcc1 的同源物,在古菌中广泛保守。Pcc1 和 Pcc2 在溶液中形成异二聚体,表现出适度的序列保守性,但具有非常高的结构相似性。五亚基古菌 KEOPS 不形成二聚体,但保留了强大的 tRNA 结合和 tA 合成活性。Pcc2 可以替代 Pcc1,但由此产生的 KEOPS 复合物失活,表明这两个同源物具有不同的功能。比较序列和结构分析表明,古菌 Pcc2 和真核 Gon7 之间可能存在进化联系。我们的工作表明,Pcc2 调节 KEOPS 复合物的寡聚状态,这种特征似乎从古菌到真核生物都得到了保守。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2b30/9889334/a86eb3f1dc96/41467_2023_36210_Fig1_HTML.jpg

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