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Integration of Transcriptomics, Proteomics, and MicroRNA Analyses Reveals Novel MicroRNA Regulation of Targets in the Mammalian Inner Ear

机译:转录组学,蛋白质组学和MicroRNA分析的整合揭示了哺乳动物内耳中靶标的新型MicroRNA调控。

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摘要

We have employed a novel approach for the identification of functionally important microRNA (miRNA)-target interactions, integrating miRNA, transcriptome and proteome profiles and advanced in silico analysis using the FAME algorithm. Since miRNAs play a crucial role in the inner ear, demonstrated by the discovery of mutations in a miRNA leading to human and mouse deafness, we applied this approach to microdissected auditory and vestibular sensory epithelia. We detected the expression of 157 miRNAs in the inner ear sensory epithelia, with 53 miRNAs differentially expressed between the cochlea and vestibule. Functionally important miRNAs were determined by searching for enriched or depleted targets in the transcript and protein datasets with an expression consistent with the dogma of miRNA regulation. Importantly, quite a few of the targets were detected only in the protein datasets, attributable to regulation by translational suppression. We identified and experimentally validated the regulation of PSIP1-P75, a transcriptional co-activator previously unknown in the inner ear, by miR-135b, in vestibular hair cells. Our findings suggest that miR-135b serves as a cellular effector, involved in regulating some of the differences between the cochlear and vestibular hair cells.
机译:我们采用了一种新颖的方法来鉴定功能上重要的microRNA(miRNA)-靶标相互作用,整合了miRNA,转录组和蛋白质组图谱,并使用FAME算法对计算机进行了高级计算机分析。由于miRNA在导致人和小鼠耳聋的miRNA突变中的发现证明了miRNA在内耳中起着至关重要的作用,因此我们将这种方法应用于显微解剖的听觉和前庭感觉上皮细胞。我们检测到内耳感觉上皮细胞中有157个miRNA的表达,其中在耳蜗和前庭之间有53个miRNA差异表达。通过在转录物和蛋白质数据集中搜索富集或耗竭的靶标来确定功能重要的miRNA,这些靶标的表达与miRNA调节的教条一致。重要的是,仅在蛋白质数据集中检测到许多靶标,这归因于翻译抑制的调控。我们鉴定并通过实验验证了miR-135b在前庭毛细胞中对PSIP1-P75(一种以前在内耳中未知的转录共激活因子)的调节。我们的发现表明,miR-135b可作为细胞效应子,参与调节耳蜗和前庭毛细胞之间的某些差异。

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