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Circ_0004535/miR-1827/CASP8 网络参与 2 型糖尿病伴非酒精性脂肪性肝病。

Circ_0004535/miR-1827/CASP8 network involved in type 2 diabetes mellitus with nonalcoholic fatty liver disease.

机构信息

Graduate School of Xinjiang Medical University, Xinshi District, Ürümqi, 830054, China.

B Chao Room, The Sixth Affiliated Hospital of Xinjiang Medical University, Tianshan District, Ürümqi, 830092, China.

出版信息

Sci Rep. 2023 Nov 13;13(1):19807. doi: 10.1038/s41598-023-47189-3.

DOI:10.1038/s41598-023-47189-3
PMID:37957232
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC10643362/
Abstract

Diagnostic delay in type 2 diabetes mellitus (T2DM) with nonalcoholic fatty liver disease (NAFLD) patients often leads to a serious public health problem. Understanding the pathophysiological mechanisms of disease will help develop more effective treatments. High-throughput sequencing was used to determine the expression levels of circRNAs, and mRNAs in health controls, T2DM patients, and T2DM with NAFLD patients. Differentially expressed genes (DEcircRs, DEmRs) in T2DM with NAFLD were identified by differential analysis. The miRNAs with targeted relationship with the DEcircRs and DEmRs were respectively predicted to construct a ceRNA regulatory network. In addition, enrichment analysis of DEmRs in the ceRNA network was performed. The expression of important DEcircRs was further validated by quantitative real-time PCR (qRT-PCR). The steatosis was detected in glucose treated LO2 cells by overexpressing circ_0004535, and CASP8. There were 586 DEmRs, and 10 DEcircRs in both T2DM and T2DM with NAFLD patients. Combined with predicted results and differential analysis, the ceRNA networks were constructed. The DEmRs in the ceRNA networks were mainly enriched in Toll-like receptor signaling pathway, and apoptosis. Importantly, dual luciferase experiments validated the targeted binding of hsa_circ_0004535 and hsa-miR-1827 or hsa-miR-1827 and CASP8. qRT-PCR experiments validated that hsa_circ_0004535, and CASP8 was downregulated and hsa-miR-1827 was upregulated expression in peripheral blood of T2DM with NAFLD patients. Abnormal cell morphology, and increased lipid droplet fusion were observed in the glucose treated LO2 cells, overexpression of circ_0004535 and CASP8 ameliorated these changes. Our work provides a deeper understanding of ceRNA mediated pathogenesis of T2DM with NAFLD and provides a novel strategy for treatment.

摘要

2 型糖尿病伴非酒精性脂肪性肝病(T2DM)患者的诊断延迟常常导致严重的公共卫生问题。了解疾病的病理生理机制将有助于开发更有效的治疗方法。使用高通量测序来确定健康对照、T2DM 患者和 T2DM 伴 NAFLD 患者中 circRNAs 和 mRNAs 的表达水平。通过差异分析确定 T2DM 伴 NAFLD 中的差异表达基因(DEcircRs、DEmRs)。分别预测与 DEcircRs 和 DEmRs 具有靶向关系的 miRNAs,以构建 ceRNA 调控网络。此外,对 ceRNA 网络中的 DEmRs 进行了富集分析。通过定量实时 PCR(qRT-PCR)进一步验证了重要 DEcircRs 的表达。通过过表达 circ_0004535 和 CASP8 来检测葡萄糖处理的 LO2 细胞中的脂肪变性。在 T2DM 和 T2DM 伴 NAFLD 患者中均存在 586 个 DEmRs 和 10 个 DEcircRs。结合预测结果和差异分析,构建了 ceRNA 网络。ceRNA 网络中的 DEmRs 主要富集在 Toll 样受体信号通路和细胞凋亡中。重要的是,双荧光素酶实验验证了 hsa_circ_0004535 与 hsa-miR-1827 或 hsa-miR-1827 与 CASP8 的靶向结合。qRT-PCR 实验验证了 hsa_circ_0004535、CASP8 在 T2DM 伴 NAFLD 患者的外周血中表达下调,hsa-miR-1827 表达上调。在葡萄糖处理的 LO2 细胞中观察到异常的细胞形态和增加的脂滴融合,过表达 circ_0004535 和 CASP8 改善了这些变化。我们的工作深入了解了 T2DM 伴 NAFLD 的 ceRNA 介导发病机制,并为治疗提供了新的策略。

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