使用 l-RNA 合体捕获 RNA G-四重结构。

IF 4.2 Q2 BIOCHEMISTRY & MOLECULAR BIOLOGY
Sin Yu Lam, Mubarak Ishaq Umar, Haizhou Zhao, Jieyu Zhao and Chun Kit Kwok
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引用次数: 0

摘要

G-quadruplexes (dG4 和 rG4)是由某些富含 G 的序列自组装形成的核酸二级结构,它们具有独特的化学特性,在基本生物过程中发挥着关键作用。研究表明,小分子 G4 配体对于确定 G4 的特性和了解其功能至关重要。然而,人们对这些合成配体在进一步研究 G4s(特别是用于分离 rG4)方面的特异性表示担忧。与 G4 配体相比,我们提出了一种新型的基于磁珠的 pulldown 检测方法,利用功能化的 l-Apt.4-1c 从简单的缓冲液和复杂的介质(包括总 RNA 和细胞裂解液)中选择性地捕获一般的 rG4s。我们发现,与 G4 小分子配体 BioTASQ v.1 相比,在非目标竞争者(包括 dG4 和非 G4 结构)存在的情况下,我们的 l-RNA aptamer 能以更高的效率和特异性牵引一般 rG4。我们的研究结果表明,生物素化的 l-aptamers 可以作为有效的分子工具,利用这种新的检测方法对感兴趣的 rG4 进行基于亲和力的富集,并通过内源转录本的定量反转录聚合酶链反应(RT-qPCR)进行了验证。这项工作为使用功能化l-aptamer分离rG4提供了新的重要见解,将来有可能应用于转录本特异性或整个转录本组。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Capture of RNA G-quadruplex structures using an l-RNA aptamer†

Capture of RNA G-quadruplex structures using an l-RNA aptamer†

Capture of RNA G-quadruplex structures using an l-RNA aptamer†

G-quadruplexes (dG4 and rG4) are nucleic acid secondary structures formed by the self-assembly of certain G-rich sequences, and they have distinctive chemical properties and play crucial roles in fundamental biological processes. Small molecule G4 ligands were shown to be crucial in characterizing G4s and understanding their functions. Nevertheless, concerns regarding the specificity of these synthetic ligands for further investigation of G4s, especially for rG4 isolation purposes, have been raised. In comparison to G4 ligands, we propose a novel magnetic bead-based pulldown assay that enables the selective capture of general rG4s using functionalized L-Apt.4-1c from both simple buffer and complex media, including total RNA and the cell lysate. We found that our L-RNA aptamer can pulldown general rG4s with a higher efficiency and specificity than the G4 small molecule ligand BioTASQ v.1 in the presence of non-target competitors, including dG4 and non-G4 structures. Our findings reveal that biotinylated L-aptamers can serve as effective molecular tools for the affinity-based enrichment of rG4 of interest using this new assay, which was also verified by quantitative reverse transcription-polymerase chain reaction (RT-qPCR) on endogenous transcripts. This work provides new and important insights into rG4 isolation using a functionalized L-aptamer, which can potentially be applied in a transcript-specific or transcriptome-wide manner in the future.

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来源期刊
CiteScore
6.10
自引率
0.00%
发文量
128
审稿时长
10 weeks
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