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哺乳动物Nudix酶在带帽RNA分析中的应用。

Application of Mammalian Nudix Enzymes to Capped RNA Analysis.

作者信息

Lukaszewicz Maciej

机构信息

Department of Biophysics, Faculty of Physics, University of Warsaw, Pasteura 5, 02-093 Warsaw, Poland.

出版信息

Pharmaceuticals (Basel). 2024 Sep 11;17(9):1195. doi: 10.3390/ph17091195.

Abstract

Following the success of mRNA vaccines against COVID-19, mRNA-based therapeutics have now become a great interest and potential. The development of this approach has been preceded by studies of modifications found on mRNA ribonucleotides that influence the stability, translation and immunogenicity of this molecule. The 5' cap of eukaryotic mRNA plays a critical role in these cellular functions and is thus the focus of intensive chemical modifications to affect the biological properties of in vitro-prepared mRNA. Enzymatic removal of the 5' cap affects the stability of mRNA in vivo. The NUDIX hydrolase Dcp2 was identified as the first eukaryotic decapping enzyme and is routinely used to analyse the synthetic cap at the 5' end of RNA. Here we highlight three additional NUDIX enzymes with known decapping activity, namely Nudt2, Nudt12 and Nudt16. These enzymes possess a different and some overlapping activity towards numerous 5' RNA cap structures, including non-canonical and chemically modified ones. Therefore, they appear as potent tools for comprehensive in vitro characterisation of capped RNA transcripts, with special focus on synthetic RNAs with therapeutic activity.

摘要

继新冠病毒mRNA疫苗取得成功之后,基于mRNA的疗法如今已引发了极大的关注并展现出巨大潜力。在这种方法的发展之前,已有关于mRNA核糖核苷酸上修饰的研究,这些修饰会影响该分子的稳定性、翻译和免疫原性。真核mRNA的5'帽在这些细胞功能中起关键作用,因此是影响体外制备mRNA生物学特性的密集化学修饰的重点。酶促去除5'帽会影响mRNA在体内的稳定性。NUDIX水解酶Dcp2被鉴定为首个真核去帽酶,常被用于分析RNA 5'端的合成帽。在此,我们重点介绍另外三种具有已知去帽活性的NUDIX酶,即Nudt2、Nudt12和Nudt16。这些酶对众多5' RNA帽结构具有不同且部分重叠的活性,包括非经典和化学修饰的结构。因此,它们似乎是对加帽RNA转录本进行全面体外表征的有力工具,尤其侧重于具有治疗活性的合成RNA。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7139/11434898/9f5854d8fa37/pharmaceuticals-17-01195-g001.jpg

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