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膝关节骨关节炎患者滑液液体部分的RNA表达谱分析

RNA expression profiling from the liquid fraction of synovial fluid in knee joint osteoarthritis patients.

作者信息

Jiang Peng, Sun Shui, Zhang Ju, Li Cuidan, Ma Guannan, Wang Jian, Chen Fei, Liao Dezhong Joshua

机构信息

School of Clinical Medicine, Shandong University Jinan 250100, Shandong Province, China.

Department of Orthopaedics, Shandong Provincial Hospital Affiliated to Shandong University Jinan 250021, Shandong Province, China.

出版信息

Am J Transl Res. 2022 Sep 15;14(9):6782-6791. eCollection 2022.

Abstract

OBJECTIVE

To investigate the RNA profile of synovial fluid (SF) from osteoarthritis (OA) patients and carry out cluster analysis of OA-related genes.

METHODS

RNA of SF from OA patients was isolated using RNA-specific Trizol. A cDNA library was built and subjected to the second-generation sequencing using HisSeq4000 with a data size of 8G. The sequencing reads were aligned to the UCSC human reference genome (hg38) using Tophat with default parameters. Gene function enrichment was generated using DAVID.

RESULTS

The minimum weight 0.096 µg RNA of SF sample was used for sequencing analysis, which produced 66,154,562 clean reads, 91.28% of which were matched to the reference with 2,682 genes identified. Some of the unmatchable reads matched RNAs of bacteria, mainly . The detected human RNAs in samples fell into different categories of genes, including protein-coding ones, processed and unprocessed pseudogenes, and long noncoding, antisense and miscellaneous RNAs that mediate various biological functions. Interestingly, 80% of the expressed genes belonged to the mitochondrial genome.

CONCLUSION

These results suggest that less than 0.1 µg RNA is sufficient for establishing a cDNA library and deep sequencing, and that the liquid fraction of SF contains a whole RNA repertoire that may reflect a history of previous microorganism infections.

摘要

目的

研究骨关节炎(OA)患者滑液(SF)的RNA谱,并对OA相关基因进行聚类分析。

方法

使用RNA特异性Trizol从OA患者的SF中分离RNA。构建cDNA文库,并使用HisSeq4000进行第二代测序,数据量为8G。使用Tophat将测序读数与UCSC人类参考基因组(hg38)进行比对,参数设置为默认值。使用DAVID进行基因功能富集分析。

结果

SF样本中最低重量为0.096μg的RNA用于测序分析,产生了66,154,562条clean reads,其中91.28%与参考基因组匹配,共鉴定出2,682个基因。一些无法匹配的读数与细菌的RNA匹配,主要是……样本中检测到的人类RNA分为不同的基因类别,包括蛋白质编码基因、加工和未加工的假基因,以及介导各种生物学功能的长链非编码RNA、反义RNA和其他RNA。有趣的是,80%的表达基因属于线粒体基因组。

结论

这些结果表明,少于0.1μg的RNA足以建立cDNA文库并进行深度测序,并且SF的液体部分包含一个完整的RNA库,可能反映了先前微生物感染的历史。

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本文引用的文献

1
Epidemiology of osteoarthritis: literature update.骨关节炎的流行病学:文献更新。
Curr Opin Rheumatol. 2018 Mar;30(2):160-167. doi: 10.1097/BOR.0000000000000479.

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