玻璃体 microRNA 在视网膜疾病中的生物标记潜力:荟萃分析

Diana Joseph, Brian Grover, Michael Telias
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引用次数: 0

摘要

增殖性糖尿病视网膜病变和老年性黄斑变性等后天性视网膜疾病给诊断和预后带来了巨大挑战。玻璃体液位于晶状体后的眼球后房中,与视网膜内部关系密切。在这种环境中,视网膜细胞分泌出多种多样的生物分子,其中可能蕴藏着重要的生物标志物。其中,短小的非编码微 RNA(miRNA)成为有希望的候选者。它们受各种基因信号转导机制的动态调控,具有更强的抗降解能力,并通过独立的外泌途径进行分泌,因此具有特别重要的意义。玻璃体 miRNA 图谱的变化可能反映病理状态,并为疾病的病因学和进展提供洞察力。我们对 22 项同行评审研究进行了全面的荟萃分析,以评估玻璃体 miRNA 作为视网膜疾病生物标记物的潜力。我们的分析表明了 miRNA 作为特定视网膜病变生物标志物的潜在作用。我们的研究表明,miR-142、miR-9 和 miR-21 是强有力的候选生物标记物,它们与增殖性玻璃体视网膜疾病有着一致且显著的相关变化。我们还探讨了表征玻璃体 miRNA 含量所面临的方法学挑战,包括缺乏标准化的纯化、扩增和分析方案,以及缺乏真正的对照样本。此外,我们还提出了采用特定的看家基因和数据归一化技术来规范玻璃体内 miRNA 分析的理由,并探讨了从健康人体内获取玻璃体样本的潜在方法。玻璃体miRNA有望成为各种视网膜疾病的潜在生物标记物,其中miR-142、miR-9和miR-21尤其具有潜力。改进玻璃体取样和 miRNA 分析方法为扩大 miRNA 生物标志物在视网膜疾病诊断和预后中的种类和用途提供了机会。
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Biomarker potential of vitreous microRNA in retinal disease: a meta-analysis
Acquired retinal diseases such as proliferative diabetic retinopathy and age-related macular degeneration pose significant challenges in diagnosis and prognosis. The vitreous fluid, situated in the posterior chamber of the eye behind the lens, holds a close relationship with the inner retina. Within this milieu, retinal cells secrete a diverse array of biomolecules, potentially harboring vital biomarkers. Among these, short, non-coding micro-RNAs (miRNAs) emerge as promising candidates. Their dynamic regulation by various gene signaling mechanisms, enhanced resistance to degradation, and secretion via separate exocytotic pathways make them particularly significant. Alterations in vitreal miRNA profiles may reflect pathological states and offer insights into disease etiology and progression. We conducted a comprehensive meta-analysis of 22 peer-reviewed studies to assess the potential of vitreous miRNAs as biomarkers for retinal diseases. Our analysis demonstrates the potential utility of miRNAs as biomarkers in specific retinal pathologies. We show that miR-142, miR-9, and miR-21 emerge as robust biomarker candidates, displaying consistent and significant alterations correlating with proliferative vitreoretinal diseases. We also address the methodological challenges encountered in characterizing vitreous miRNA content, including the absence of standardized purification, amplification, and analysis protocols, as well as the scarcity of true control samples. Moreover, we make the case for the adoption of specific housekeeping genes and data normalization techniques to standardize miRNA analysis in the vitreous and explore potential methodologies for obtaining vitreous samples from healthy individuals. Vitreous miRNAs hold promise as potential biomarkers for various retinal diseases, with miR-142, miR-9, and miR-21 emerging as particularly promising candidates. Enhancing methodologies for vitreous sampling and miRNA analysis presents an opportunity to expand the repertoire and utility of miRNA biomarkers in retinal disease diagnosis and prognosis.
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