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Identification of a novel cis-acting RNA element involved in nuclear export of hY RNAs.

机译:鉴定涉及hY RNA核输出的新型顺式作用RNA元件。

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摘要

Ro RNPs are small cytoplasmic RNA-protein complexes of unknown function that have been found in all metazoan cells studied so far. In human cells, Ro RNPs consist of one of four small RNA molecules, termed hY RNAs and at least two well-characterized proteins, Ro60 and La. In previous Xenopus laevis oocyte microinjection studies, we showed that an intact Ro60 binding site (Stem-loop 1) is a prerequisite for efficient nuclear export of hY1 RNA, whereas an intact La-binding site promotes nuclear retention (Simons et al. RNA, 1996, 2:264-273). Here we present evidence that the distal half (Stem 2) of the conserved base-paired stem structure found in all hY RNAs also plays a critical role in the export process. A minimal RNA molecule containing this region, L1S2 RNA, competes effectively for the export of full-length hY1 RNAs and is itself exported very rapidly in a Ro60-independent and RanGTP-dependent manner. Mutational analyses of this RNA shows that a 5'/3' terminal double-stranded stem structure (>10 bp) of no specific nucleotide sequence constitutes a novel nuclear export element (NEE). Cross-competition studies indicate that this type of NEE may also be involved in export of other classes of RNAs. Like full-length hY1 RNA, L1S2 RNA also competes for export of ET-202 RNA, an RNA that was selected for its efficient nuclear export in the presence of the nuclear transport inhibitor, VSV Matrix protein (Grimm et al. Proc Natl Acad Sci USA, 1997, 94:10122-10127). However, export of L1S2 RNA is strongly inhibited by VSV-M protein, showing that these RNAs use partially overlapping, but not identical export pathways. We propose that export of Y RNAs is mediated by two contiguous cis-acting elements in the 5'/3' double-stranded stem region that is conserved between different Y RNAs.
机译:Ro RNP是迄今在所有研究的后生细胞中发现的功能未知的小细胞质RNA-蛋白质复合物。在人类细胞中,Ro RNP由四个小RNA分子之一(称为hY RNA)和至少两个特征明确的蛋白质Ro60和La组成。在以前的非洲爪蟾卵母细胞显微注射研究中,我们证明了完整的Ro60结合位点(Stem-环1)是hY1 RNA有效核输出的先决条件,而完整的La结合位点可促进核保留(Simons等,RNA,1996,2:264-273)。在这里,我们提供的证据表明,在所有hY RNA中发现的保守碱基对茎结构的远端一半(第2茎)在出口过程中也起着至关重要的作用。包含此区域的最小RNA分子L1S2 RNA可有效竞争全长hY1 RNA的输出,并且自身以Ro60独立和RanGTP依赖的方式非常快速地输出。该RNA的突变分析表明,没有特定核苷酸序列的5'/ 3'末端双链茎结构(> 10 bp)构成了新的核输出元件(NEE)。交叉竞争研究表明,这种NEE也可能参与其他类别RNA的输出。与全长hY1 RNA一样,L1S2 RNA也竞争ET-202 RNA的输出,ET-202 RNA是在存在核转运抑制剂VSV Matrix蛋白的情况下被选择用于有效核输出的RNA(Grimm等,Proc Natl Acad Sci美国,1997,94:10122-10127)。但是,VSV-M蛋白强烈抑制L1S2 RNA的输出,表明这些RNA使用部分重叠但不相同的输出途径。我们建议,Y RNA的出口是由5'/ 3'双链茎区域中两个连续的顺式作用元件介导的,而这两个区域在不同的Y RNA之间是保守的。

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