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Possible role of microRNA miRNA-IL-25 interaction in mice with ulcerative colitis

机译:MicroRNA miRNA-IL-25与溃疡性结肠炎小鼠相互作用的可能作用

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摘要

Background: The regulatory network of ulcerative colitis (UC)-associated miRNAs is not fully understood. In this study, we aim to investigate the global profile and regulatory network of UC associated miRNAs in the context of dextran sulfate sodium (DSS). Methods: UC was induced in C57BL mice using DSS. Differentially expressed miRNAs were screened by RNA sequencing and subjected to the Kyoto Encyclopedia of Genes and Genomes Pathway enrichment analysis. RT-qPCR was used to verify the differential expression of miRNAs and candidate target mRNA. Luciferase reporter vector bearing a miRNA binding site was constructed to verify the binding site of the miRNA on mRNA. Results:A total of 95 miRNAs (31 were up-regulated and 64 were down regulated) differentially expressed in the colonic tissues of the UC mice. Among the differentially expressed miRNAs, IL-25 pathway genes were enriched. Subsequent RT-qPCR confirmed a decreased expression of IL-25 and a significant up regulation of IL-25 target miRNAs including mmu-miR-135b-5p, mmu-miR-7239-5p and mmu-miR-691 in UC mice. Conclusion: Using the luciferase assay, we verified the biding sites of mmu-miR-135b-5p and mmu-miR-691 to the IL-25 3ʹUTR. In conclusion, mmu-miR-135b-5p:IL-25 and mmu-miR-691:IL-25 interactions are important pathways that may exert a protective role in UC.
机译:背景:溃疡性结肠炎(UC)的调节网络尤其是分类的miRNA不完全理解。在这项研究中,我们的目标是在葡聚糖硫酸钠(DSS)的背景下研究UC相关miRNA的全局概况和调节网络。方法:使用DSS在C57BL小鼠中诱导UC。通过RNA测序筛选差异表达的miRNA,并进行基因的京都群细胞和基因组途径富集分析。 RT-QPCR用于验证miRNA和候选靶mRNA的差异表达。构建轴承MiRNA结合位点的荧光素酶报告载体以验证miRNA对mRNA的结合位点。结果:在UC小鼠的结肠组织中,总共95个miRNA(31次上调,64次被调节)。在差异表达的miRNA中,富集IL-25途径基因。随后的RT-QPCR证实了IL-25的表达降低和IL-25靶MiRNA的显着调节,包括UC小鼠的MMU-MIR-135B-5P,MMU-MIR-7239-5P和MMU-MIR-691。结论:使用荧光素酶测定,验证了MMU-MIR-135B-5P和MMU-MIR-691的弯曲部位至IL-25 3'UTR。总之,MMU-MIR-135B-5P:IL-25和MMU-MIR-691:IL-25相互作用是可能在UC中发挥保护作用的重要途径。

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