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In-gel probing of individual RNA conformers within a mixed population reveals a dimerization structural switch in the HIV-1 leader

机译:混合人群中单个RNA构象体的凝胶内探测揭示了HIV-1前导分子的二聚化结构转换

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Definitive secondary structural mapping of RNAs in vitro can be complicated by the presence of more than one structural conformer or multimerization of some of the molecules. Until now, probing a single structure of conformationally flexible RNA molecules has typically relied on introducing stabilizing mutations or adjusting buffer conditions or RNA concentration. Here, we present an in-gel SHAPE (selective 2'OH acylation analysed by primer extension) approach, where a mixed structural population of RNA molecules is separated by non-denaturing gel electrophoresis and the conformers are individually probed within the gel matrix. Validation of the technique using a well-characterized RNA stem-loop structure, the HIV-1 trans-activation response element, showed that authentic structure was maintained and that the method was accurate and highly reproducible. To further demonstrate the utility of in-gel SHAPE, we separated and examined monomeric and dimeric species of the HIV-1 packaging signal RNA. Extensive differences in acylation sensitivity were seen between monomer and dimer. The results support a recently proposed structural switch model of RNA genomic dimerization and packaging, and demonstrate the discriminatory power of in-gel SHAPE.
机译:RNA的体外确定性二级结构作图可能会由于存在一个以上的结构构象异构体或某些分子发生多聚化而变得复杂。到目前为止,探测构象柔性RNA分子的单个结构通常依赖于引入稳定突变或调节缓冲液条件或RNA浓度。在这里,我们提出了凝胶内SHAPE(通过引物延伸分析选择性2'OH酰化)方法,其中RNA分子的混合结构群通过非变性凝胶电泳分离,并且构象体在凝胶基质中单独检测。使用特征明确的RNA茎环结构,HIV-1反式激活应答元件对该技术进行的验证表明,该结构得以保留,并且该方法准确且可重复性高。为了进一步证明凝胶内SHAPE的实用性,我们分离并检查了HIV-1包装信号RNA的单体和二聚体种类。在单体和二聚体之间观察到酰化敏感性的广泛差异。结果支持最近提出的RNA基因组二聚化和包装的结构转换模型,并证明了凝胶内SHAPE的区分能力。

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