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Drosha 切割编码 miR-10b 和 HOXD4 的转录本产生的未加帽 RNA 的核积累。

Nuclear accumulation of an uncapped RNA produced by Drosha cleavage of a transcript encoding miR-10b and HOXD4.

机构信息

School of Biological Sciences, Nanyang Technological University, Singapore.

出版信息

PLoS One. 2011;6(10):e25689. doi: 10.1371/journal.pone.0025689. Epub 2011 Oct 3.

Abstract

Patterning of the animal embryo's antero-posterior (AP) axis is dependent on spatially and temporally regulated Hox gene expression. The murine Hoxd4 gene has been proposed to harbour two promoters, an upstream promoter P2, and a downstream promoter P1, that lie 5.2 and 1.1 kilobase pairs (kb) upstream of the coding region respectively. The evolutionarily conserved microRNA-10b (miR-10b) gene lies in the Hoxd4 genomic locus in the intron separating the non-coding exons 4 and 5 of the P2 transcript and directly adjacent to the proposed P1 promoter. Hoxd4 transcription is regulated by a 3' neural enhancer that harbours a retinoic acid response element (RARE). Here, we show that the expression profiles of Hoxd4 and miR-10b transcripts during neural differentiation of mouse embryonal carcinoma (EC) P19 cells are co-ordinately regulated, suggesting that both Hoxd4 and miR-10b expression is governed by the neural enhancer. Our observation that P1 transcripts are uncapped, together with the mapping of their 5' ends, strongly suggests that they are generated by Drosha cleavage of P2 transcripts rather than by transcriptional initiation. This is supported by the colocalization of P1 and P2 transcripts to the same posterior expression domain in the mouse embryo. These uncapped P1 transcripts do not appear to possess an Internal Ribosomal Entry Site (IRES), but accumulate within multiple punctate bodies within the nucleus suggesting that they play a functional role. Finally, similar uncapped Drosha-cleaved P1-like transcripts originating from the paralogous Hoxb4/miR-10a locus were also identified. We propose that these transcripts may belong to a novel class of regulatory RNAs.

摘要

动物胚胎的前-后(AP)轴的模式形成依赖于时空调节的 Hox 基因表达。鼠 Hoxd4 基因被提出具有两个启动子,上游启动子 P2 和下游启动子 P1,分别位于编码区上游 5.2 和 1.1 千碱基对(kb)处。进化上保守的 microRNA-10b(miR-10b)基因位于 Hoxd4 基因组基因座内,位于 P2 转录物的非编码外显子 4 和 5 之间的内含子中,并且直接毗邻所提出的 P1 启动子。Hoxd4 转录受 3'神经增强子调节,该增强子包含视黄酸反应元件(RARE)。在这里,我们表明在小鼠胚胎癌细胞(EC)P19 细胞的神经分化过程中,Hoxd4 和 miR-10b 转录物的表达谱是协调调节的,这表明 Hoxd4 和 miR-10b 的表达均受神经增强子控制。我们观察到 P1 转录物未加帽,并且其 5'端进行了映射,这强烈表明它们是由 P2 转录物的 Drosha 切割产生的,而不是由转录起始产生的。这得到了 P1 和 P2 转录物在小鼠胚胎中聚集到相同的后表达域的结果的支持。这些未加帽的 P1 转录物似乎不具有内部核糖体进入位点(IRES),但在核内的多个点状体内积累,这表明它们发挥了功能作用。最后,还鉴定了来自同源基因座 Hoxb4/miR-10a 的类似未加帽的 Drosha 切割的 P1 样转录物。我们提出这些转录物可能属于一类新的调节 RNA。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a6fc/3185001/237203734d98/pone.0025689.g001.jpg

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