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A Spinach molecular beacon triggered by strand displacement

机译:链位移触发的菠菜分子信标

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摘要

We have re-engineered the fluorescent RNA aptamer Spinach to be activated in a sequence-dependent manner. The original Spinach aptamer was extended at its 5′- and 3′-ends to create Spinach.ST, which is predicted to fold into an inactive conformation and thus prevent association with the small molecule fluorophore DFHBI. Hybridization of a specific trigger oligonucleotide to a designed toehold leads to toehold-initiated strand displacement and refolds Spinach into the active, fluorophore-binding conformation. Spinach.ST not only specifically detects its target oligonucleotide but can discriminate readily against single-nucleotide mismatches. RNA amplicons produced during nucleic acid sequence-based amplification (NASBA) of DNA or RNA targets could be specifically detected and reported in real-time by conformational activation of Spinach.ST generated by in vitro transcription. In order to adapt any target sequence to detection by a Spinach reporter we used a primer design technique that brings together otherwise distal toehold sequences via hairpin formation. The same techniques could potentially be used to adapt common Spinach reporters to non-nucleic acid analytes, rather than by making fusions between aptamers and Spinach.
机译:我们已经重新设计了荧光RNA适体菠菜,以序列依赖性方式激活。最初的菠菜适体在其5'-和3'-末端延伸以生成Spinach.ST,预计可折叠成非活性构象,从而防止与小分子荧光团DFHBI缔合。特定触发寡核苷酸与设计的鞋头的杂交会导致鞋头引发的链置换,并使菠菜重折叠成具有活性的荧光团结合构象。 Spinach.ST不仅可以特异性地检测其靶寡核苷酸,而且可以轻松区分单核苷酸错配。通过体外转录产生的Spinach.ST的构象激活,可以特异性检测和实时报告DNA或RNA靶标的基于核酸序列的扩增(NASBA)过程中产生的RNA扩增子。为了使任何靶序列适应于菠菜报道分子的检测,我们使用了引物设计技术,该技术通过发夹形成将远端的脚趾序列聚集在一起。相同的技术可能会潜在地用于使普通Spinach报告基因适应非核酸分析物,而不是通过在适体和Spinach之间融合来实现。

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