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延伸因子P(EF-P)及其旁系同源物EfpL(YeiP)对含脯氨酸序列的翻译具有不同的调控作用。

EF-P and its paralog EfpL (YeiP) differentially control translation of proline-containing sequences.

作者信息

Sieber Alina, Parr Marina, von Ehr Julian, Dhamotharan Karthikeyan, Kielkowski Pavel, Brewer Tess, Schäpers Anna, Krafczyk Ralph, Qi Fei, Schlundt Andreas, Frishman Dmitrij, Lassak Jürgen

机构信息

Faculty of Biology, Microbiology, Ludwig-Maximilians-Universität München, Planegg-Martinsried, Germany.

Department of Bioinformatics, Wissenschaftszentrum Weihenstephan, Technische Universität München, Freising, Germany.

出版信息

Nat Commun. 2024 Dec 2;15(1):10465. doi: 10.1038/s41467-024-54556-9.

Abstract

Polyproline sequences are deleterious to cells because they stall ribosomes. In bacteria, EF-P plays an important role in overcoming such polyproline sequence-induced ribosome stalling. Additionally, numerous bacteria possess an EF-P paralog called EfpL (also known as YeiP) of unknown function. Here, we functionally and structurally characterize EfpL from Escherichia coli and demonstrate its role in the translational stress response. Through ribosome profiling, we analyze the EfpL arrest motif spectrum and find additional sequences beyond the canonical polyproline motifs that both EF-P and EfpL can resolve. Notably, the two factors can also induce pauses. We further report that EfpL can sense the metabolic state of the cell via lysine acylation. Overall, our work characterizes the role of EfpL in ribosome rescue at proline-containing sequences, and provides evidence that co-occurrence of EF-P and EfpL is an evolutionary driver for higher bacterial growth rates.

摘要

多聚脯氨酸序列对细胞有害,因为它们会使核糖体停滞。在细菌中,延伸因子P(EF-P)在克服此类多聚脯氨酸序列诱导的核糖体停滞方面发挥着重要作用。此外,许多细菌拥有一种名为EfpL(也称为YeiP)的EF-P旁系同源物,其功能未知。在这里,我们对来自大肠杆菌的EfpL进行了功能和结构表征,并证明了其在翻译应激反应中的作用。通过核糖体分析,我们分析了EfpL的停滞基序谱,并发现了除了EF-P和EfpL都能解决的典型多聚脯氨酸基序之外的其他序列。值得注意的是,这两种因子也会诱导停顿。我们进一步报道,EfpL可以通过赖氨酸酰化感知细胞的代谢状态。总体而言,我们的工作表征了EfpL在含脯氨酸序列的核糖体拯救中的作用,并提供了证据表明EF-P和EfpL的共存是细菌更高生长速率的进化驱动力。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/59a9/11611912/6a480caf0ddf/41467_2024_54556_Fig1_HTML.jpg

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