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类风湿关节炎患者血浆长链非编码RNA表达谱

Plasma Long Non-Coding RNA Expression Profiles in Patients with Rheumatoid Arthritis.

作者信息

Qin Wen, Wang Ting-Hui, Xie Bin-Hua, Sun Qing-Qing, Huang Hua, Zhao Bao-Jing, Cen Han, Wu Xiu-Di

出版信息

Clin Lab. 2019 Aug 1;65(8). doi: 10.7754/Clin.Lab.2019.190144.

DOI:10.7754/Clin.Lab.2019.190144
PMID:31414744
Abstract

BACKGROUND

Recently, long non-coding RNAs (lncRNAs) have attracted substantial attention owing to their unforeseen critical roles in a wide range of biological processes. The aim of our study was to provide an overview of lncRNA expression profiles in plasma of RA patients.

METHODS

The Agilent LncRNA + mRNA Human Gene Expression Microarray V4.0 was employed to determine differentially expressed (DE) lncRNAs and mRNAs in plasma of four female newly diagnosed and DMARD-naïve RA patients and four female age-matched healthy controls. The KOBAS (KEGG Orthology Based Annotation System) software was applied to determine the gene ontology (GO) terms and pathway in which the DE mRNAs were enriched. Furthermore, a lncRNA-mRNA co-expression network was constructed according to the correlation between DE lncRNAs and mRNAs.

RESULTS

Compared with healthy controls, a total of 289 DE lncRNAs (169 up-regulated and 120 down-regulated) and 468 DE mRNAs (280 up-regulated and 188 down-regulated) were found in the plasma of patients with RA. Bioinformatics analysis indicated that the DE mRNAs might be involved in the pathogenesis of RA mainly through platelets. In addition, a co-expression network composed of 229 network nodes and 340 connections between 116 lncRNAs and 113 mRNAs was constructed.

CONCLUSIONS

We characterized the plasma lncRNA expression profiles in RA patients for the first time. Our results could shed new light on the pathogenesis of RA and help identify lncRNAs as novel diagnostic biomarkers and therapeutic targets for RA.

摘要

背景

最近,长链非编码RNA(lncRNA)因其在广泛生物过程中发挥的意外关键作用而备受关注。我们研究的目的是概述类风湿关节炎(RA)患者血浆中lncRNA的表达谱。

方法

使用安捷伦lncRNA + mRNA人类基因表达微阵列V4.0来确定4名新诊断且未使用改善病情抗风湿药(DMARD)的女性RA患者和4名年龄匹配的女性健康对照者血浆中差异表达的(DE)lncRNA和mRNA。应用KOBAS(基于KEGG直系同源注释系统)软件来确定DE mRNA富集的基因本体(GO)术语和通路。此外,根据DE lncRNA与mRNA之间的相关性构建lncRNA-mRNA共表达网络。

结果

与健康对照相比,在RA患者血浆中总共发现了289个DE lncRNA(169个上调和120个下调)和468个DE mRNA(280个上调和188个下调)。生物信息学分析表明,DE mRNA可能主要通过血小板参与RA的发病机制。此外,构建了一个由229个网络节点以及116个lncRNA与113个mRNA之间的340个连接组成的共表达网络。

结论

我们首次对RA患者血浆中的lncRNA表达谱进行了表征。我们的结果可为RA的发病机制提供新的线索,并有助于将lncRNA鉴定为RA的新型诊断生物标志物和治疗靶点。

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