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变形链球菌中多样化的 A-to-I 编辑的动态变化受 mRNA 稳定性的改变所调控。

Dynamics of diversified A-to-I editing in Streptococcus pyogenes is governed by changes in mRNA stability.

机构信息

Max Planck Unit for the Science of Pathogens, 10117 Berlin, Germany.

Institute for Biology, Humboldt University Berlin, 10115 Berlin, Germany.

出版信息

Nucleic Acids Res. 2024 Oct 14;52(18):11234-11253. doi: 10.1093/nar/gkae629.

Abstract

Adenosine-to-inosine (A-to-I) RNA editing plays an important role in the post-transcriptional regulation of eukaryotic cell physiology. However, our understanding of the occurrence, function and regulation of A-to-I editing in bacteria remains limited. Bacterial mRNA editing is catalysed by the deaminase TadA, which was originally described to modify a single tRNA in Escherichia coli. Intriguingly, several bacterial species appear to perform A-to-I editing on more than one tRNA. Here, we provide evidence that in the human pathogen Streptococcus pyogenes, tRNA editing has expanded to an additional tRNA substrate. Using RNA sequencing, we identified more than 27 editing sites in the transcriptome of S. pyogenes SF370 and demonstrate that the adaptation of S. pyogenes TadA to a second tRNA substrate has also diversified the sequence context and recoding scope of mRNA editing. Based on the observation that editing is dynamically regulated in response to several infection-relevant stimuli, such as oxidative stress, we further investigated the underlying determinants of editing dynamics and identified mRNA stability as a key modulator of A-to-I editing. Overall, our findings reveal the presence and diversification of A-to-I editing in S. pyogenes and provide novel insights into the plasticity of the editome and its regulation in bacteria.

摘要

腺嘌呤到次黄嘌呤(A-to-I)RNA 编辑在真核细胞生理的转录后调控中发挥着重要作用。然而,我们对细菌中 A-to-I 编辑的发生、功能和调控的理解仍然有限。细菌 mRNA 编辑由脱氨酶 TadA 催化,该酶最初被描述为修饰大肠杆菌中的单个 tRNA。有趣的是,几种细菌似乎在不止一种 tRNA 上进行 A-to-I 编辑。在这里,我们提供的证据表明,在人类病原体酿脓链球菌中,tRNA 编辑已经扩展到另一种 tRNA 底物。通过 RNA 测序,我们在酿脓链球菌 SF370 的转录组中鉴定出超过 27 个编辑位点,并证明酿脓链球菌 TadA 对第二种 tRNA 底物的适应也使 mRNA 编辑的序列背景和重编码范围多样化。基于观察到编辑是动态调节的,以响应几种感染相关的刺激,如氧化应激,我们进一步研究了编辑动态的潜在决定因素,并确定 mRNA 稳定性是 A-to-I 编辑的关键调节剂。总的来说,我们的研究结果揭示了酿脓链球菌中 A-to-I 编辑的存在和多样化,并为细菌中 editome 的可塑性及其调控提供了新的见解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/be18/11472039/3323de73aa6e/gkae629figgra1.jpg

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