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尽管人类反转录转座子 RNA 的基因组插入机制相同,但它们在细胞内的分布是离散的。

Discrete subcellular partitioning of human retrotransposon RNAs despite a common mechanism of genome insertion.

机构信息

Department of Genetics, University of Pennsylvania School of Medicine, Philadelphia, PA 19104, USA.

出版信息

Hum Mol Genet. 2010 May 1;19(9):1712-25. doi: 10.1093/hmg/ddq048. Epub 2010 Feb 10.

DOI:10.1093/hmg/ddq048
PMID:20147320
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2850619/
Abstract

Despite the immense significance retrotransposons have had for genome evolution much about their biology is unknown, including the processes of forming their ribonucleoprotein (RNP) particles and transporting them about the cell. Suppression of retrotransposon expression, together with the presence of retrotransposon sequence within numerous mRNAs, makes tracking endogenous L1 RNP particles in cells problematic. We overcame these difficulties by assaying in living and fixed cells tagged-RNPs generated from constructs expressing retrotransposition-competent L1s. In this way, we demonstrate for the first time the subcellular colocalization of L1 RNA and proteins ORF1p and ORF2p, and show their targeting together to cytoplasmic foci. Foci are often associated with markers of cytoplasmic stress granules. Furthermore, mutation analyses reveal that ORF1p can direct L1 RNP distribution within the cell. We also assayed RNA localization of the non-autonomous retrotransposons Alu and SVA. Despite a requirement for the L1 integration machinery, each manifests unique features of subcellular RNA distribution. In nuclei Alu RNA forms small round foci partially associated with marker proteins for coiled bodies, suborganelles involved in the processing of non-coding RNAs. SVA RNA patterning is distinctive, being cytoplasmic but without prominent foci and concentrated in large nuclear aggregates that often ring nucleoli. Such variability predicts significant differences in the life cycles of these elements.

摘要

尽管逆转录转座子在基因组进化中具有重要意义,但它们的许多生物学特性仍不为人知,包括形成核糖核蛋白 (RNP) 颗粒和在细胞内运输的过程。逆转录转座子表达的抑制以及大量 mRNA 中存在逆转录转座子序列,使得追踪细胞内内源性 L1 RNP 颗粒成为一个问题。我们通过检测表达具有逆转座活性的 L1 的构建体中产生的标记-RNP 来克服这些困难。通过这种方式,我们首次证明了 L1 RNA 和蛋白质 ORF1p 和 ORF2p 的亚细胞共定位,并显示它们一起靶向细胞质焦点。焦点通常与细胞质应激颗粒的标志物相关。此外,突变分析表明,ORF1p 可以指导 L1 RNP 在细胞内的分布。我们还检测了非自主逆转录转座子 Alu 和 SVA 的 RNA 定位。尽管需要 L1 整合机制,但每个都表现出亚细胞 RNA 分布的独特特征。在核内,Alu RNA 形成小的圆形焦点,部分与参与非编码 RNA 加工的卷曲体标记蛋白相关联,卷曲体是参与非编码 RNA 加工的亚细胞器。SVA RNA 的模式是独特的,它位于细胞质中,但没有明显的焦点,并且集中在经常环绕核仁的大核聚集体中。这种可变性预测了这些元素生命周期的显著差异。

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本文引用的文献

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5'-Transducing SVA retrotransposon groups spread efficiently throughout the human genome.5'-转导 SVA 逆转录转座子群有效地在人类基因组中扩散。
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Exon-trapping mediated by the human retrotransposon SVA.由人类反转录转座子 SVA 介导的外显子捕获。
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Diverse cis factors controlling Alu retrotransposition: what causes Alu elements to die?控制Alu逆转录转座的多种顺式作用因子:是什么导致Alu元件失活?
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Active Alu retrotransposons in the human genome.人类基因组中的活跃Alu逆转座子。
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The Cajal body.卡哈尔体。
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