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Induction of differentiation-specific miRNAs in TPA-induced myeloid leukemia cells through MEK/ERK activation

机译:通过MEK / ERK激活诱导TPA诱导的骨髓白血病细胞中分化特异性miRNA

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Cellular microRNAs (miRNAs) are pivotal regulators involved in various biological processes through the post-transcriptional regulation of gene expression. Signaling pathways are extensively activated during 12-O-Tetradecanoylphorbol-13-acetate (TPA)-induced differentiation of human leukemia cells, but the modulation of miRNA expression and processing in this context has yet to be fully explored. In this study, we comprehensively analyzed 10?miRNAs that are consistently upregulated during TPA-induced differentiation of various leukemia cell lines by employing microarray technology. The upregulation of these miRNAs was further verified by quantitative RT-PCR, and, markedly, a subset of the miRNAs was found to be induced via the MEK/ERK signaling pathway using TPA and specific pharmacological inhibitors. Moreover, immunoblotting and quantitative RT-PCR analysis demonstrated that the expression levels of key miRNA processing machineries (i.e., Drosha, Dicer, Ago1 and Ago2) were not induced in this context, but the transcription of the miRNA products was triggered by MEK/ERK activation. Therefore, we identified the unique miRNAs that respond to TPA treatment in leukemia cells and demonstrated the essential role of the MEK/ERK signaling pathway in the induction of these miRNA transcripts.
机译:细胞microRNAs(miRNA)是通过基因表达的转录后调节涉及各种生物过程的枢转调节剂。在12-O-四癸酰基(TPA)诱导人白血病细胞的分化期间,信号传导途径被广泛激活,但在这一背景下的miRNA表达和加工的调节尚未得到充分探索。在这项研究中,我们通过采用微阵列技术综合分析了10℃的10℃,该致统计诱导的TPA诱导的各种白血病细胞系分化。通过定量RT-PCR进一步验证这些miRNA的上调,并且明显地发现MIRNA的子集通过使用TPA和特定的药理学抑制剂通过MEK / ERK信号通路诱导。此外,免疫印迹和定量RT-PCR分析表明,关键miRNA加工机械的表达水平(即Drosha,Dicer,Aga1和auga2)未在这种情况下诱导,但MiRNA产品的转录被MEK / ERK触发激活。因此,我们确定了对白血病细胞中TPA治疗的独特miRNA,并证明了MEK / ERK信号通路在这些miRNA转录物诱导中的基本作用。

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