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敲低小非编码RNA中的方法学障碍。

Methodological obstacles in knocking down small noncoding RNAs.

作者信息

Ploner Andreas, Ploner Christian, Lukasser Melanie, Niederegger Harald, Hüttenhofer Alexander

出版信息

RNA. 2009 Oct;15(10):1797-804. doi: 10.1261/rna.1740009. Epub 2009 Aug 18.

DOI:10.1261/rna.1740009
PMID:19690100
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2743047/
Abstract

In the recent past, several thousand noncoding RNA (ncRNA) genes have been predicted within eukaryal genomes. However, for their functional analysis only a few high-throughput methods are currently available to knock down selected ncRNA species, such as microRNAs, which are targeted by antisense probes, termed antagomirs. We thus compared the efficiencies of four knockdown strategies, previously mainly employed for the analysis of protein-coding genes, to study the function of ncRNAs, in particular, small nucleolar RNAs (snoRNAs). Thereby, the class of snoRNAs represents one of the most abundant ncRNA species. The majority of snoRNAs has been shown to mediate nucleotide modifications by targeting ribosomal RNAs (rRNAs) through complementary antisense elements. However, some snoRNAs, termed "orphan snoRNAs," lack telltale complementarities to rRNAs and thus their function remains elusive. We therefore applied RNA interference (RNAi), locked nucleic acid (LNA), or peptide nucleic acid antisense approaches, as well as a ribozyme-based strategy to knock down a snoRNA. As a proof of principle, we targeted the canonical U81 snoRNA, which has been shown to mediate modification of nucleotide A(391) within eukaryal 28S rRNA. Our results demonstrate that while RNAi is an unsuitable tool for snoRNA knockdown, a ribozyme-based strategy, as well as an LNA-antisense oligonucleotide approach, resulted in a decrease of U81 snoRNA expression levels up to 60%. However, no concomitant decrease in enzymatic activity of U81 snoRNA was observed, indicating that improvement of more efficient knockdown techniques for ncRNAs will be required in the future.

摘要

最近,在真核生物基因组中预测出了数千个非编码RNA(ncRNA)基因。然而,就其功能分析而言,目前仅有少数高通量方法可用于敲低选定的ncRNA种类,例如被反义探针(称为抗miR)靶向的微小RNA。因此,我们比较了四种先前主要用于蛋白质编码基因分析的敲低策略,以研究ncRNA的功能,特别是小核仁RNA(snoRNA)。snoRNA类别是最丰富的ncRNA种类之一。大多数snoRNA已被证明通过互补的反义元件靶向核糖体RNA(rRNA)来介导核苷酸修饰。然而,一些被称为“孤儿snoRNA”的snoRNA与rRNA缺乏明显的互补性,因此其功能仍然难以捉摸。因此,我们应用了RNA干扰(RNAi)、锁核酸(LNA)或肽核酸反义方法,以及基于核酶的策略来敲低一种snoRNA。作为原理验证,我们靶向了典型的U81 snoRNA,它已被证明可介导真核生物28S rRNA中核苷酸A(391)的修饰。我们的结果表明,虽然RNAi不适用于snoRNA敲低,但基于核酶的策略以及LNA反义寡核苷酸方法可使U81 snoRNA表达水平降低高达60%。然而,未观察到U81 snoRNA酶活性的相应降低,这表明未来需要改进更有效的ncRNA敲低技术。

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