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新型 RNA 聚合酶 III 启动子转录的成熟且具有功能的病毒 miRNA。

Mature and functional viral miRNAs transcribed from novel RNA polymerase III promoters.

机构信息

Program in Molecular Biology, University of Colorado Denver School of Medicine, Aurora, Colorado, 80045, USA.

出版信息

RNA. 2010 Jan;16(1):170-85. doi: 10.1261/rna.1873910. Epub 2009 Nov 30.

Abstract

Murid herpesvirus 4 (MuHV-4) microRNAs were previously cloned from latently infected tumor cells and predicted to be processed from a series of RNA polymerase III primary transcripts. We detected maturely processed MuHV-4 miRNAs within total RNA from lytically infected cells in vitro and infected tissues ex vivo, using a highly sensitive reverse ligation meditated RT-PCR strategy. We determined that the MuHV-4 microRNAs are biologically active during infection by a luciferase reporter system. We experimentally demonstrated that transcription of the MuHV-4 microRNAs is by RNA polymerase III by alpha-amanitin insensitivity and by specific deletion of the RNA polymerase III type 2-like promoter elements of MuHV-4, resulting in the complete loss of miRNA detection and function. Finally, we demonstrate that these 10 viral miRNAs, each transcribed from highly conserved and novel polymerase III promoter elements, vary markedly in their relative abundance and activity.

摘要

鼠疱疹病毒 4(MuHV-4)microRNAs 先前从潜伏感染的肿瘤细胞中克隆出来,并预测是从一系列 RNA 聚合酶 III 初级转录本中加工而来的。我们使用高度敏感的反向连接介导的 RT-PCR 策略,在体外裂解感染细胞和体外感染组织的总 RNA 中检测到成熟加工的 MuHV-4 microRNAs。我们通过荧光素酶报告系统证实 MuHV-4 microRNAs 在感染过程中具有生物活性。我们通过实验证明,MuHV-4 microRNAs 的转录是由 RNA 聚合酶 III 介导的,对 alpha-amanitin 不敏感,并且通过 MuHV-4 的 RNA 聚合酶 III 型 2 样启动子元件的特异性缺失,导致 miRNA 的检测和功能完全丧失。最后,我们证明这 10 种病毒 microRNAs ,分别由高度保守和新型 RNA 聚合酶 III 启动子元件转录而来,其相对丰度和活性差异显著。

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