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对染色质上 hnRNP A2/B1-RNA 结合的全局分析突出了 LncRNA 相互作用。

Global profiling of hnRNP A2/B1-RNA binding on chromatin highlights LncRNA interactions.

机构信息

a Molecular Biology Program , University of Colorado Denver Anschutz Medical Campus , Aurora , CO , USA.

b Department of Biochemistry and Molecular Genetics, Aurora , University of Colorado School of Medicine , CO , USA.

出版信息

RNA Biol. 2018;15(7):901-913. doi: 10.1080/15476286.2018.1474072. Epub 2018 Jul 25.

Abstract

Long noncoding RNAs (lncRNAs) often carry out their functions through associations with adaptor proteins. We recently identified heterogeneous ribonucleoprotein (hnRNP) A2/B1 as an adaptor of the human HOTAIR lncRNA. hnRNP A2 and B1 are splice isoforms of the same gene. The spliced version of HOTAIR preferentially associates with the B1 isoform, which we hypothesize contributes to RNA-RNA matching between HOTAIR and transcripts of target genes in breast cancer. Here we used enhanced cross-linking immunoprecipitation (eCLIP) to map the direct interactions between A2/B1 and RNA in breast cancer cells. Despite differing by only twelve amino acids, the A2 and B1 splice isoforms associate preferentially with distinct populations of RNA in vivo. Through cellular fractionation experiments we characterize the pattern of RNA association in chromatin, nucleoplasm, and cytoplasm. We find that a majority of interactions occur on chromatin, even those that do not contribute to co-transcriptional splicing. A2/B1 binding site locations on multiple RNAs hint at a contribution to the regulation and function of lncRNAs. Surprisingly, the strongest A2/B1 binding site occurs in a retained intron of HOTAIR, which interrupts an RNA-RNA interaction hotspot. In vitro eCLIP experiments highlight additional exonic B1 binding sites in HOTAIR which also surround the RNA-RNA interaction hotspot. Interestingly, a version of HOTAIR with the intron retained is still capable of making RNA-RNA interactions in vitro through the hotspot region. Our data further characterize the multiple functions of a repurposed splicing factor with isoform-biased interactions, and highlight that the majority of these functions occur on chromatin-associated RNA.

摘要

长链非编码 RNA(lncRNA)通常通过与衔接蛋白的相互作用来发挥其功能。我们最近发现异质核糖核蛋白(hnRNP)A2/B1 是人类 HOTAIR lncRNA 的衔接蛋白。hnRNP A2 和 B1 是同一基因的剪接异构体。HOTAIR 的剪接版本优先与 B1 异构体结合,我们假设这有助于 HOTAIR 与乳腺癌靶基因转录本之间的 RNA-RNA 匹配。在这里,我们使用增强交联免疫沉淀(eCLIP)来绘制乳腺癌细胞中 A2/B1 与 RNA 之间的直接相互作用。尽管仅相差十二个氨基酸,A2 和 B1 剪接异构体在体内仍优先与不同的 RNA 群体结合。通过细胞分级分离实验,我们对染色质、核质和细胞质中 RNA 的结合模式进行了表征。我们发现,大多数相互作用发生在染色质上,即使那些不参与共转录剪接的相互作用也是如此。多个 RNA 上的 A2/B1 结合位点位置暗示了它们对 lncRNA 的调节和功能的贡献。令人惊讶的是,最强的 A2/B1 结合位点出现在 HOTAIR 中一个保留的内含子中,该内含子中断了 RNA-RNA 相互作用的热点。体外 eCLIP 实验突出了 HOTAIR 中额外的 B1 结合外显子位点,这些位点也环绕着 RNA-RNA 相互作用热点。有趣的是,保留内含子的 HOTAIR 版本仍然能够通过热点区域在体外进行 RNA-RNA 相互作用。我们的数据进一步描述了具有异构体偏向性相互作用的重新利用剪接因子的多种功能,并强调这些功能中的大多数发生在染色质相关 RNA 上。

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