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福司可林通过 hnRNP K 控制神经元分化中的可变剪接。

Control of alternative splicing by forskolin through hnRNP K during neuronal differentiation.

机构信息

Department of Physiology, University of Manitoba, Winnipeg, MB R3E 0J9, Canada.

出版信息

Nucleic Acids Res. 2012 Sep;40(16):8059-71. doi: 10.1093/nar/gks504. Epub 2012 Jun 8.

DOI:10.1093/nar/gks504
PMID:22684629
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3439897/
Abstract

The molecular basis of cell signal-regulated alternative splicing at the 3' splice site remains largely unknown. We isolated a protein kinase A-responsive ribonucleic acid (RNA) element from a 3' splice site of the synaptosomal-associated protein 25 (Snap25) gene for forskolin-inhibited splicing during neuronal differentiation of rat pheochromocytoma PC12 cells. The element binds specifically to heterogeneous nuclear ribonucleo protein (hnRNP) K in a phosphatase-sensitive way, which directly competes with the U2 auxiliary factor U2AF65, an essential component of early spliceosomes. Transcripts with similarly localized hnRNP K target motifs upstream of alternative exons are enriched in genes often associated with neurological diseases. We show that such motifs upstream of the Runx1 exon 6 also bind hnRNP K, and importantly, hnRNP K is required for forskolin-induced repression of the exon. Interestingly, this exon encodes the peptide domain that determines the switch of the transcriptional repressor/activator activity of Runx1, a change known to be critical in specifying neuron lineages. Consistent with an important role of the target genes in neurons, knocking down hnRNP K severely disrupts forskolin-induced neurite growth. Thus, through hnRNP K, the neuronal differentiation stimulus forskolin targets a critical 3' splice site component of the splicing machinery to control alternative splicing of crucial genes. This also provides a regulated direct competitor of U2AF65 for cell signal control of 3' splice site usage.

摘要

细胞信号调控 3' 剪接位点选择性剪接的分子基础在很大程度上仍是未知的。我们从突触相关蛋白 25 (Snap25) 基因的 3' 剪接位点分离出一个蛋白激酶 A 反应性核糖核酸 (RNA) 元件,用于分离福司可林抑制神经分化大鼠嗜铬细胞瘤 PC12 细胞中的剪接。该元件以磷酸酶敏感的方式特异性结合异质核核糖核蛋白 (hnRNP) K,直接与早期剪接体的必需成分 U2 辅助因子 U2AF65 竞争。具有类似定位 hnRNP K 靶标基序的转录本在上游的替代外显子中富集,这些基因通常与神经疾病有关。我们表明,Runx1 外显子 6 上游的类似基序也与 hnRNP K 结合,重要的是,hnRNP K 是福司可林诱导该外显子抑制所必需的。有趣的是,该外显子编码决定转录抑制物/激活剂活性的 Runx1 肽结构域的切换,这种变化在确定神经元谱系方面是至关重要的。与靶基因在神经元中的重要作用一致,敲低 hnRNP K 严重破坏了福司可林诱导的轴突生长。因此,通过 hnRNP K,神经元分化刺激福司可林靶向剪接机制的关键 3' 剪接位点成分,以控制关键基因的选择性剪接。这也为 U2AF65 的细胞信号控制 3' 剪接位点使用提供了一种受调控的直接竞争物。

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