Ravi Bhushan, A. Rani, D. Gupta, Akhtar Ali, P. Dubey
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Further, target genes were verified in-vitro through transfection and RT-qPCR.\n\n\nRESULTS\nFive miRNAs, namely hsa-let 7a-5P, hsa-miR7-5P, hsa-miR9-5P, hsa-miR18a-5P, and hsa-miR23a-3P were significantly over-expressed (p < 0.05) in all three samples namely PL, CB, and MB of GDM patients. However, the sample-wise comparison reveals higher expression of miRNA 7 in MB while lowest in CB than control. Furthermore, a comparison of fold change expression of target genes discloses a lower expression of IRS1, IRS2, and RAF1 in MB while comparatively higher expression of NRAS in MB and CB. In-vitro validation reveals lower expression of IRS1/2 and RAF1 in response to overexpression of miR-7 and vice-versa. Thus it is evident that increased miRNA7 expression causes down-regulation of its target genes IRS1, IRS2, and RAF1 in GDM mother compared to control. Further, target prediction, pathway enrichment, and hormone analysis (significantly higher FSH & LH in MB of GDM compared to NGT) revealed the insulin signaling, inflammatory and GnRH signaling as major pathways regulated by miRNA7.\n\n\nCONCLUSIONS\nThus, an elevated level of miRNA7 may be associated with the progression of GDM by altering the multiple pathways like insulin, GnRH, and inflammatory signaling pathways via targeting IRS1, IRS2, and RAF1, implicating a new therapeutic target for GDM.","PeriodicalId":38067,"journal":{"name":"MicroRNA (Shariqah, United Arab Emirates)","volume":"1 1","pages":""},"PeriodicalIF":0.0000,"publicationDate":"2022-04-13","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"5","resultStr":"{\"title\":\"MicroRNA-7 regulates insulin signaling pathway by targeting IRS1, IRS2, and RAF1 genes in gestational diabetes mellitus.\",\"authors\":\"Ravi Bhushan, A. Rani, D. Gupta, Akhtar Ali, P. 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引用次数: 5
摘要
小的非编码微rna (miRNAs)参与多种代谢过程,并在包括妊娠糖尿病(GDM)在内的疾病病理中发挥关键作用。目的研究非糖耐量(NGT)和GDM配对的母亲胎盘组织(PL)、脐带血(CB)和母体血(MB)中miRNAs及其靶基因的表达变化。方法采用茎环RT-qPCR方法,对45例血清(MB n = 15, CB n = 15, PL n = 15)和匹配胎盘组织的微rna进行定量分析,并进行靶标预测、网络构建、功能和途径富集分析。进一步,通过转染和RT-qPCR对靶基因进行体外验证。结果hsa-let 7a-5P、hsa-miR7-5P、hsa-miR9-5P、hsa-miR18a-5P、hsa-miR23a-3P 5种mirna在GDM患者PL、CB和MB中均显著过表达(p < 0.05)。然而,样本比较显示,miRNA - 7在MB中的表达高于对照组,而在CB中的表达低于对照组。此外,通过比较靶基因的折叠变化表达,发现MB中IRS1、IRS2和RAF1的表达较低,而MB和CB中NRAS的表达相对较高。体外验证显示,miR-7过表达会导致IRS1/2和RAF1的低表达,反之亦然。由此可见,在GDM母鼠中,miRNA7表达增加导致其靶基因IRS1、IRS2和RAF1较对照下调。此外,靶标预测、途径富集和激素分析(GDM的MB中FSH和LH明显高于NGT)显示,胰岛素信号、炎症和GnRH信号是miRNA7调节的主要信号通路。因此,miRNA7水平升高可能通过靶向IRS1、IRS2和RAF1改变胰岛素、GnRH和炎症信号通路等多种途径与GDM的进展相关,提示GDM的新治疗靶点。
MicroRNA-7 regulates insulin signaling pathway by targeting IRS1, IRS2, and RAF1 genes in gestational diabetes mellitus.
BACKGROUND
Small non-coding micro RNAs (miRNAs) are indicated in various metabolic processes and play a critical role in disease pathology, including gestational diabetes mellitus (GDM).
OBJECTIVE
The purpose of this study was to examine the altered expression of miRNAs and their target genes in placental tissue (PL), cord blood (CB), and maternal blood (MB) of matched non-glucose tolerant (NGT) and GDM mother.
METHODS
In a case-control study, micro-RNA was quantified from forty-five serum (MB n = 15, CB n = 15, and PL n = 15) and matched placental tissue using stem-loop RT-qPCR followed by target prediction, network construction and functional and pathways enrichment analysis. Further, target genes were verified in-vitro through transfection and RT-qPCR.
RESULTS
Five miRNAs, namely hsa-let 7a-5P, hsa-miR7-5P, hsa-miR9-5P, hsa-miR18a-5P, and hsa-miR23a-3P were significantly over-expressed (p < 0.05) in all three samples namely PL, CB, and MB of GDM patients. However, the sample-wise comparison reveals higher expression of miRNA 7 in MB while lowest in CB than control. Furthermore, a comparison of fold change expression of target genes discloses a lower expression of IRS1, IRS2, and RAF1 in MB while comparatively higher expression of NRAS in MB and CB. In-vitro validation reveals lower expression of IRS1/2 and RAF1 in response to overexpression of miR-7 and vice-versa. Thus it is evident that increased miRNA7 expression causes down-regulation of its target genes IRS1, IRS2, and RAF1 in GDM mother compared to control. Further, target prediction, pathway enrichment, and hormone analysis (significantly higher FSH & LH in MB of GDM compared to NGT) revealed the insulin signaling, inflammatory and GnRH signaling as major pathways regulated by miRNA7.
CONCLUSIONS
Thus, an elevated level of miRNA7 may be associated with the progression of GDM by altering the multiple pathways like insulin, GnRH, and inflammatory signaling pathways via targeting IRS1, IRS2, and RAF1, implicating a new therapeutic target for GDM.
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