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Stem-loop RNA labeling can affect nuclear and cytoplasmic mRNA processing

机译:茎环RNA标记会影响核和细胞质mRNA加工

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The binding of sequence-specific RNA-interacting proteins, such as the bacteriophage MS2 or PP7 coat proteins, to their corresponding target sequences has been extremely useful and widely used to visualize single mRNAs in vivo. However, introduction of MS2 stem-loops into yeast mRNAs has recently been shown to lead to the accumulation of RNA fragments, suggesting that the loops impair mRNA decay. This result was questioned, because fragment occurrence was mainly assessed using ensemble methods, and their cellular localization and its implications had not been addressed on a single transcript level. Here, we demonstrate that the introduction of either MS2 stem-loops (MS2SL) or PP7 stem loops (PP7SL) can affect the processing and subcellular localization of mRNA. We use single-molecule fluorescence in situ hybridization (smFISH) to determine the localization of three independent mRNAs tagged with the stem loop labeling systems in glucose-rich and glucose starvation conditions. Transcripts containing MS2SL or PP7SL display aberrant localization in both the nucleus and the cytoplasm. These defects are most prominent in glucose starvation conditions, with nuclear mRNA processing being altered and stem-loop fragments abnormally enriching in processing bodies (PBs). The mislocalization of SL-containing RNAs is independent of the presence of the MS2 or PP7 coat protein (MCP or PCP).
机译:序列特异性RNA相互作用的蛋白质(例如噬菌体MS2或PP7涂层蛋白)的结合对于它们的相应靶序列非常有用,并且广泛用于在体内可视化单个MRNA。然而,最近被证明将MS2茎环引入酵母mRNAs以导致RNA片段的积累,这表明环损伤损伤。该结果质疑,因为主要使用集合方法评估片段发生,并且它们的细胞定位及其含义尚未在单个转录水平上进行解决。这里,我们证明了MS2茎环(MS2S1)或PP7茎环(PP7SL)的引入可以影响mRNA的处理和亚细胞定位。我们使用原位杂交(SMFISH)的单分子荧光来确定三个独立MRNA的定位标记,所述三个独立的MRNA标记为猪环标记系统,富含葡萄糖和葡萄糖饥饿条件。含有MS2S1或PP7SL的转录物在细胞核和细胞质中显示异常定位。这些缺陷在葡萄糖饥饿条件下最突出,核mRNA处理被改变,并且在加工体中异常富集的茎环片段(PBS)。含有SL的RNA的错误定位与MS2或PP7涂层蛋白(MCP或PCP)的存在无关。

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