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首页> 外文期刊>Investigative ophthalmology & visual science >MicroRNA Profiling in Aqueous Humor of Individual Human Eyes by Next-Generation Sequencing
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MicroRNA Profiling in Aqueous Humor of Individual Human Eyes by Next-Generation Sequencing

机译:通过下一代测序对人眼的幽默进行MicroRNA分析

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Purpose: Extracellular microRNAs (miRNAs) in aqueous humor were suggested to have a role in transcellular signaling and may serve as disease biomarkers. The authors adopted next-generation sequencing (NGS) techniques to further characterize the miRNA profile in single samples of 60 to 80 ??L human aqueous humor. Methods: Samples were obtained at the outset of cataract surgery in nine independent, otherwise healthy eyes. Four samples were used to extract RNA and generate sequencing libraries, followed by an adapter-driven amplification step, electrophoretic size selection, sequencing, and data analysis. Five samples were used for quantitative PCR (qPCR) validation of NGS results. Published NGS data on circulating miRNAs in blood were analyzed in comparison. Results: One hundred fifty-eight miRNAs were consistently detected by NGS in all four samples; an additional 59 miRNAs were present in at least three samples. The aqueous humor miRNA profile shows some overlap with published NGS-derived inventories of circulating miRNAs in blood plasma with high prevalence of human miR-451a, -21, and -16. In contrast to blood, miR-184, -4448, -30a, -29a, -29c, -19a, -30d, -205, -24, -22, and -3074 were detected among the 20 most prevalent miRNAs in aqueous humor. Relative expression patterns of miR-451a, -202, and -144 suggested by NGS were confirmed by qPCR. Conclusions: Our data illustrate the feasibility of miRNA analysis by NGS in small individual aqueous humor samples. Intraocular cells as well as blood plasma contribute to the extracellular aqueous humor miRNome. The data suggest possible roles of miRNA in intraocular cell adhesion and signaling by TGF-?2 and Wnt, which are important in intraocular pressure regulation and glaucoma.
机译:目的:房水中的细胞外微小RNA(miRNA)被认为在跨细胞信号传导中起作用,并可能充当疾病的生物标记。作者采用了下一代测序(NGS)技术来进一步表征60至80μL人房水的单个样品中的miRNA谱。方法:在白内障手术开始时,从9只独立的健康眼睛中获得样本。使用四个样品提取RNA并生成测序文库,然后进行适配器驱动的扩增步骤,电泳大小选择,测序和数据分析。将五个样品用于NGS结果的定量PCR(qPCR)验证。比较分析了已发布的有关血液中循环miRNA的NGS数据。结果:NGS在所有四个样本中均一致地检测到了158个miRNA。至少三个样品中还存在59个miRNA。房水miRNA谱显示与血浆中循环的miRNA的已发表的NGS衍生清单有些重叠,其中人类miR-451a,-21和-16的患病率很高。与血液相反,在房水中的20种最流行的miRNA中检测到miR-184,-4448,-30a,-29a,-29c,-19a,-30d,-205,-24,-22和-3074 。通过qPCR证实了NGS提出的miR-451a,-202和-144的相对表达模式。结论:我们的数据说明了在较小的单个房水样本中通过NGS分析miRNA的可行性。眼内细胞以及血浆有助于细胞外房水miRNome。数据表明miRNA可能通过TGF-β2和Wnt在眼内细胞粘附和信号传导中发挥作用,这在眼内压调节和青光眼中很重要。

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