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环状 RNA 丰富、保守,并与 ALU 重复序列相关。

Circular RNAs are abundant, conserved, and associated with ALU repeats.

机构信息

Department of Genetics, University of North Carolina School of Medicine, Chapel Hill, North Carolina 27599-7295, USA.

出版信息

RNA. 2013 Feb;19(2):141-57. doi: 10.1261/rna.035667.112. Epub 2012 Dec 18.

Abstract

Circular RNAs composed of exonic sequence have been described in a small number of genes. Thought to result from splicing errors, circular RNA species possess no known function. To delineate the universe of endogenous circular RNAs, we performed high-throughput sequencing (RNA-seq) of libraries prepared from ribosome-depleted RNA with or without digestion with the RNA exonuclease, RNase R. We identified >25,000 distinct RNA species in human fibroblasts that contained non-colinear exons (a "backsplice") and were reproducibly enriched by exonuclease degradation of linear RNA. These RNAs were validated as circular RNA (ecircRNA), rather than linear RNA, and were more stable than associated linear mRNAs in vivo. In some cases, the abundance of circular molecules exceeded that of associated linear mRNA by >10-fold. By conservative estimate, we identified ecircRNAs from 14.4% of actively transcribed genes in human fibroblasts. Application of this method to murine testis RNA identified 69 ecircRNAs in precisely orthologous locations to human circular RNAs. Of note, paralogous kinases HIPK2 and HIPK3 produce abundant ecircRNA from their second exon in both humans and mice. Though HIPK3 circular RNAs contain an AUG translation start, it and other ecircRNAs were not bound to ribosomes. Circular RNAs could be degraded by siRNAs and, therefore, may act as competing endogenous RNAs. Bioinformatic analysis revealed shared features of circularized exons, including long bordering introns that contained complementary ALU repeats. These data show that ecircRNAs are abundant, stable, conserved and nonrandom products of RNA splicing that could be involved in control of gene expression.

摘要

circRNA 是由外显子序列组成的环状 RNA,在少数基因中被描述过。人们认为,circRNA 是由剪接错误产生的,它们没有已知的功能。为了描绘内源性 circRNA 的宇宙,我们对核糖体耗尽的 RNA 进行了高通量测序(RNA-seq),这些 RNA 来自用或不用 RNA 外切酶 RNase R 处理的文库。我们在人类成纤维细胞中鉴定出了超过 25000 种独特的 RNA 物种,这些 RNA 包含非共线性外显子(“回文剪接”),并且可以通过线性 RNA 的外切酶降解来重现富集。这些 RNA 被验证为环状 RNA(circRNA),而不是线性 RNA,并且在体内比相关的线性 mRNA 更稳定。在某些情况下,环状分子的丰度比相关的线性 mRNA 高出 10 倍以上。保守估计,我们在人类成纤维细胞中活跃转录的基因中鉴定出了 14.4%的 circRNA。将这种方法应用于小鼠睾丸 RNA,鉴定出了在人类 circRNA 中精确同源的位置的 69 个 circRNA。值得注意的是,平行激酶 HIPK2 和 HIPK3 在人和小鼠的第二个外显子中产生大量的 circRNA。虽然 HIPK3 circRNA 包含一个 AUG 翻译起始,但它和其他 circRNA 没有与核糖体结合。circRNA 可以被 siRNA 降解,因此可能作为竞争内源性 RNA 发挥作用。生物信息学分析揭示了环状外显子的共同特征,包括含有互补 ALU 重复的长边界内含子。这些数据表明,circRNA 是 RNA 剪接的丰富、稳定、保守和非随机产物,可能参与基因表达的调控。

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