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长读长RNA测序揭示了等位基因特异性N6-甲基腺苷修饰。

Long-read RNA sequencing reveals allele-specific -methyladenosine modifications.

作者信息

Park Dayea, Cenik Can

机构信息

Department of Molecular Biosciences, University of Texas at Austin, Austin, Texas 78712, USA.

Department of Molecular Biosciences, University of Texas at Austin, Austin, Texas 78712, USA

出版信息

Genome Res. 2025 Apr 14;35(4):999-1011. doi: 10.1101/gr.279270.124.

Abstract

Long-read sequencing technology enables highly accurate detection of allele-specific RNA expression, providing insights into the effects of genetic variation on splicing and RNA abundance. Furthermore, the ability to directly sequence RNA enables the detection of RNA modifications in tandem with ascertaining the allelic origin of each molecule. Here, we leverage these advantages to determine allele-biased patterns of -methyladenosine (mA) modifications in native mRNA. We used human and mouse cells with known genetic variants to assign the allelic origin of each mRNA molecule combined with a supervised machine learning model to detect read-level mA modification ratios. Our analyses reveal the importance of sequences adjacent to the DRACH motif in determining mA deposition, in addition to allelic differences that directly alter the motif. Moreover, we discover allele-specific mA modification events with no genetic variants in close proximity to the differentially modified nucleotide, demonstrating the unique advantage of using long-reads and surpassing the capabilities of antibody-based short-read approaches. This technological advance will further our understanding of the role of genetics in determining mRNA modifications.

摘要

长读长测序技术能够高度准确地检测等位基因特异性RNA表达,为深入了解遗传变异对剪接和RNA丰度的影响提供了线索。此外,直接对RNA进行测序的能力使得在确定每个分子的等位基因起源的同时能够检测RNA修饰。在这里,我们利用这些优势来确定天然mRNA中N6-甲基腺苷(m6A)修饰的等位基因偏向模式。我们使用具有已知遗传变异的人类和小鼠细胞来确定每个mRNA分子的等位基因起源,并结合一个监督机器学习模型来检测读段水平的m6A修饰比率。我们的分析揭示了除了直接改变基序的等位基因差异外,DRACH基序附近的序列在确定m6A沉积中的重要性。此外,我们发现了在差异修饰核苷酸附近没有紧密相邻遗传变异的等位基因特异性m6A修饰事件,证明了使用长读长的独特优势,并超越了基于抗体的短读长方法的能力。这一技术进步将进一步加深我们对遗传学在确定mRNA修饰中的作用的理解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7b7e/12047277/3ea1dbfb94a8/999f01.jpg

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