A Clustering Approach to Identify Intergenic Non-coding RNA in Mouse Macrophages

L. Garmire, S. Subramaniam, D. Garmire, C. Glass
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引用次数: 2

Abstract

We present a global clustering approach to identify putative intergenic non-coding RNAs based on the RNA polymerase II and Histone 3 lysine 4 trimethylation signatures. Both of these signatures are processed from the digital sequencing tags produced by chromatin immunoprecipitation, a high-throughput massively parallel sequencing (ChIP-Seq) technology. Our method compares favorably to the comparison method. We characterize the intergenic non-coding RNAs to have conservative promoters. We predict that these nc-RNAs are related to metabolic process without lipopolysaccharides (LPS) treatment, but shift towards developmental and immune-related functions with LPS treatment. We demonstrate that more intergenic nc-RNAs respond positively to LPS treatment, rather than negatively. Using QPCR, we experimentally validate 8 out of 11 nc-RNA regions respond to LPS treatment as predicted by the computational method.
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聚类方法鉴定小鼠巨噬细胞中基因间非编码RNA
我们提出了一种基于RNA聚合酶II和组蛋白3赖氨酸4三甲基化特征的全球聚类方法来鉴定假定的基因间非编码RNA。这两种特征都是由染色质免疫沉淀(一种高通量大规模平行测序(ChIP-Seq)技术)产生的数字测序标签处理的。我们的方法比比较法好。我们将基因间非编码rna描述为具有保守启动子。我们预测这些nc- rna在没有脂多糖(LPS)处理的情况下与代谢过程有关,但在LPS处理下转向发育和免疫相关功能。我们证明更多的基因间nc- rna对LPS处理有积极反应,而不是消极反应。使用QPCR,我们实验验证了11个nc-RNA区域中的8个响应LPS处理,正如计算方法预测的那样。
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