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人源微小RNA-483 -3p通过TGFβ2/SMAD4信号通路调控糖皮质激素反应性人小梁网细胞中的细胞外基质蛋白。

Hsa-MiR-483 -3p regulates the extracellular matrix proteins via TGFβ2/SMAD4 signaling in the glucocorticoid-responsive human trabecular meshwork cells.

作者信息

Haribalaganesh Ravinarayanan, Sharmila Rajendrababu, Krishnadas Ramasamy, Willoughby Colin E, Senthilkumari Srinivasan

机构信息

Department of Ocular Pharmacology, Aravind Medical Research Foundation, #1, Anna Nagar, Madurai, 625020, Tamilnadu, India.

Glaucoma Clinic, Aravind Eye Hospital, #1, Anna Nagar, Madurai, Tamilnadu, India.

出版信息

Cell Tissue Res. 2025 Jun 5. doi: 10.1007/s00441-025-03985-z.

DOI:10.1007/s00441-025-03985-z
PMID:40471287
Abstract

The purpose of this study was to investigate the role of hsa-miR-483-3p on the regulation of extracellular matrix (ECM) in cultured human trabecular meshwork (HTM) cells with known steroid response. Primary cultures of HTM cells with known steroid responsiveness [GC-responder (GC-R) and GC-Non-responder (GC-NR) cells] were grown on coverslip in 12-well plate until 80% confluence and treated with 100 nM dexamethasone (DEX) for 24 h and transfected with different concentrations of synthetic miRNA 483-3p mimic or inhibitor. After 24 h or 72 h post transfection, the cells were harvested for the following experiments: (i) percentage transfection efficiency, (ii) RNA isolation for qPCR analysis, (iii) immunofluorescence staining, and (iv) protein isolation for Western blotting, respectively. All experiments were performed in triplicate with three biological samples (n = 3). GC-R HTM cells showed significantly higher expression of SMAD4 as compared to GC-NR HTM cells. Similarly, DEX treatment up-regulated the SMAD4-dependent ECM proteins. The presence of a miR-483-3p mimic down-regulated SMAD4 expression and SMAD4-dependent ECM production in a dose-dependent manner by negatively down-regulating SMAD4/TGF-β2 signaling. The inhibition of SMAD4-dependent ECM production by miR-483-3p was more pronounced in GC-R HTM cells as compared to GC-NR cells. The down-regulation in ECM production by miR-483-3p is SMAD4-dependent and may play a protective role in mitigating steroid response in GC-R HTM cells. Using miR-483-3p mimics demonstrates therapeutic potential for the management of steroid-induced ocular hypertension and glaucoma.

摘要

本研究的目的是探讨hsa-miR-483-3p在已知类固醇反应的培养人小梁网(HTM)细胞中对细胞外基质(ECM)调节的作用。将具有已知类固醇反应性的HTM细胞原代培养物[糖皮质激素反应者(GC-R)和糖皮质激素无反应者(GC-NR)细胞]接种在12孔板的盖玻片上,培养至80%汇合,用100 nM地塞米松(DEX)处理24小时,并用不同浓度的合成miRNA 483-3p模拟物或抑制剂转染。转染后24小时或72小时,收获细胞用于以下实验:(i)转染效率百分比,(ii)提取RNA用于qPCR分析,(iii)免疫荧光染色,以及(iv)提取蛋白质用于蛋白质印迹分析。所有实验均重复进行三次,采用三个生物学样本(n = 3)。与GC-NR HTM细胞相比,GC-R HTM细胞中SMAD4的表达明显更高。同样,DEX处理上调了依赖SMAD4的ECM蛋白。miR-483-3p模拟物的存在通过负向下调SMAD4/TGF-β2信号,以剂量依赖的方式下调SMAD4表达和依赖SMAD4的ECM产生。与GC-NR细胞相比,miR-483-3p对依赖SMAD4的ECM产生的抑制在GC-R HTM细胞中更为明显。miR-483-3p对ECM产生的下调是依赖SMAD4的,可能在减轻GC-R HTM细胞中的类固醇反应中起保护作用。使用miR-483-3p模拟物证明了其在治疗类固醇诱导的高眼压和青光眼方面的治疗潜力。

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Upregulated MicroRNA-483-3p is an Early Event in Pancreatic Ductal Adenocarcinoma (PDAC) and as a Powerful Liquid Biopsy Biomarker in PDAC.
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