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通过蛋白质组学方法评估视网膜前膜患者玻璃体液样本中的蛋白质谱。

Assessment of protein profile in vitreous samples of patients with epiretinal membrane by proteomic approaches.

作者信息

Sumer Fatma, Ozkan Berna, Karabas V Levent, Akpinar Gurler, Kasap Murat

机构信息

Recep Tayyip Erdogan University Faculty of Medicine, Department of Ophthalmology, 53100, Rize, Turkey.

Department of Ophthalmology, Acıbadem Mehmet Ali Aydınlar University School of Medicine, İstanbul, 41100, Turkey.

出版信息

Exp Eye Res. 2025 Jan;250:110160. doi: 10.1016/j.exer.2024.110160. Epub 2024 Nov 17.

DOI:10.1016/j.exer.2024.110160
PMID:39551177
Abstract

This study aims to characterize idiopathic epiretinal membrane (iERM) using proteomic analysis to enhance diagnosis and treatment strategies. In a prospective case-control clinical trial, vitreous fluids (VF) from twelve iERM patients were collected during surgery and analyzed by 2DE-based MALDI TOF-TOF MS/MS. PANTHER and STRING analyses were performed to investigate the biological relationships between the identified proteins and to determine relevant cellular pathways. A total of 148 proteins were identified, including 24 that were unique to iERM. Grouping the proteins by biological processes revealed that most were involved in cell adhesion (n = 6), proteolysis (n = 10), and complement activation (n = 8). Compared to control VF, 12 proteins were upregulated and 12 downregulated in iERM VF, with the differentially expressed proteins strongly associated with inflammation. Proteomic analysis highlighted complement and inflammatory proteins as potential biomarkers or therapeutic targets for iERM. Given that inflammation and fibrosis play critical roles in iERM, further investigation into these differential proteins holds significant clinical relevance. Despite the challenge of recruiting suitable patients, we believe the results of this study provide a valuable foundation for future research.

摘要

本研究旨在通过蛋白质组学分析对特发性视网膜前膜(iERM)进行特征描述,以改进诊断和治疗策略。在一项前瞻性病例对照临床试验中,在手术期间收集了12例iERM患者的玻璃体液(VF),并通过基于二维电泳的基质辅助激光解吸电离飞行时间串联质谱(MALDI TOF-TOF MS/MS)进行分析。进行了PANTHER和STRING分析,以研究已鉴定蛋白质之间的生物学关系,并确定相关的细胞途径。总共鉴定出148种蛋白质,其中24种是iERM特有的。按生物学过程对蛋白质进行分组显示,大多数蛋白质参与细胞黏附(n = 6)、蛋白水解(n = 10)和补体激活(n = 8)。与对照VF相比,iERM VF中有12种蛋白质上调,12种蛋白质下调,差异表达的蛋白质与炎症密切相关。蛋白质组学分析突出了补体和炎症蛋白作为iERM潜在的生物标志物或治疗靶点。鉴于炎症和纤维化在iERM中起关键作用,对这些差异蛋白的进一步研究具有重要的临床意义。尽管招募合适患者存在挑战,但我们相信本研究结果为未来研究提供了有价值的基础。

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