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古菌 Lsm 蛋白与富含 poly(U)的靶 RNA 共转录结合。

The archaeal Lsm protein from binds co-transcriptionally to poly(U)-rich target RNAs.

机构信息

Institute of Microbiology & Archaea Centre, Single-Molecule Biochemistry Lab, University of Regensburg, D-93053 Regensburg, Germany.

Institute of Biochemistry, Genetics and Microbiology (Biochemistry I), Protein Mass Spectrometry Laboratory, University of Regensburg, D-93053 Regensburg, Germany.

出版信息

Biol Chem. 2023 Sep 15;404(11-12):1085-1100. doi: 10.1515/hsz-2023-0215. Print 2023 Oct 26.

DOI:10.1515/hsz-2023-0215
PMID:37709673
Abstract

Posttranscriptional processes in Bacteria include the association of small regulatory RNAs (sRNA) with a target mRNA. The sRNA/mRNA annealing process is often mediated by an RNA chaperone called Hfq. The functional role of bacterial and eukaryotic Lsm proteins is partially understood, whereas knowledge about archaeal Lsm proteins is scarce. Here, we used the genetically tractable archaeal hyperthermophile to identify the protein interaction partners of the archaeal Sm-like proteins (PfuSmAP1) using mass spectrometry and performed a transcriptome-wide binding site analysis of PfuSmAP1. Most of the protein interaction partners we found are part of the RNA homoeostasis network in Archaea including ribosomal proteins, the exosome, RNA-modifying enzymes, but also RNA polymerase subunits, and transcription factors. We show that PfuSmAP1 preferentially binds messenger RNAs and antisense RNAs recognizing a gapped poly(U) sequence with high affinity. Furthermore, we found that SmAP1 co-transcriptionally associates with target RNAs. Our study reveals that in contrast to bacterial Hfq, PfuSmAP1 does not affect the transcriptional activity or the pausing behaviour of archaeal RNA polymerases. We propose that PfuSmAP1 recruits antisense RNAs to target mRNAs and thereby executes its putative regulatory function on the posttranscriptional level.

摘要

细菌中的转录后过程包括小调控 RNA(sRNA)与靶 mRNA 的结合。sRNA/mRNA 退火过程通常由一种称为 Hfq 的 RNA 伴侣介导。细菌和真核生物 Lsm 蛋白的功能作用部分得到了解,而古菌 Lsm 蛋白的知识则相对较少。在这里,我们使用遗传上可操作的古菌嗜热菌来鉴定古菌 Sm 样蛋白(PfuSmAP1)的蛋白相互作用伙伴,使用质谱法,并对 PfuSmAP1 的转录组进行了广泛的结合位点分析。我们发现的大多数蛋白相互作用伙伴都是古菌 RNA 稳态网络的一部分,包括核糖体蛋白、外切体、RNA 修饰酶,但也包括 RNA 聚合酶亚基和转录因子。我们表明,PfuSmAP1 优先结合信使 RNA 和反义 RNA,识别具有高亲和力的缺口多聚(U)序列。此外,我们发现 SmAP1 与靶 RNA 共转录相关。我们的研究表明,与细菌 Hfq 不同,PfuSmAP1 不会影响古菌 RNA 聚合酶的转录活性或暂停行为。我们提出,PfuSmAP1 将反义 RNA 招募到靶 mRNA 上,从而在转录后水平上执行其潜在的调节功能。

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