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RNA double cleavage by a hairpin-derived twin ribozyme.

机译:发夹衍生的双核酶对RNA的双重切割。

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The hairpin ribozyme is a small catalytic RNA that catalyses reversible sequence-specific RNA hydrolysis in trans. It consists of two domains, which interact with each other by docking in an antiparallel fashion. There is a region between the two domains acting as a flexible hinge for interdomain interactions to occur. Hairpin ribozymes with reverse-joined domains have been constructed by dissecting the domains at the hinge and rejoining them in reverse order. We have used both the conventional and reverse-joined hairpin ribozymes for the design of a hairpin-derived twin ribozyme. We show that this twin ribozyme cleaves a suitable RNA substrate at two specific sites while maintaining the target specificity of the individual monoribozymes. For characterisation of the studied ribozymes we have evaluated a quantitative assay of sequence-specific ribozyme activity using fluorescently labelled RNA substrates in conjunction with an automated DNA sequencer. This assay was found to be applicable with hairpin and hairpin-derived ribozymes. The results demonstrate the potential of hairpin ribozymes for multi-target strategies of RNA cleavage and suggest the possibility for employing hairpin-derived twin ribozymes as powerful tools for RNA manipulation in vitro and in vivo.
机译:发夹状核酶是一种小的催化RNA,可催化反式可逆的序列特异性RNA水解。它由两个域组成,这两个域通过以反平行方式对接而彼此交互。在两个域之间存在一个区域,充当域间交互作用发生的灵活铰链。具有反向连接结构域的发夹状核酶已通过在铰链处解剖结构域并以相反顺序将其重新连接而构建。我们已经使用了传统的和反向连接的发夹状核酶进行发夹衍生的双核酶的设计。我们显示该双核酶在两个特定位点切割合适的RNA底物,同时保持单个核糖核酸酶的靶标特异性。为了表征所研究的核酶,我们评估了使用荧光标记的RNA底物结合自动DNA测序仪对序列特异性核酶活性进行定量测定的方法。发现该测定法适用于发夹和发夹衍生的核酶。结果证明了发夹状核酶在RNA切割的多目标策略中的潜力,并暗示了将发夹状双核酶作为体外和体内RNA操纵的强大工具的可能性。

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