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Sensitive and label-free biosensing of RNA with predicted secondary structures by a triplex affinity capture method

机译:通过三重亲和力捕获方法对具有预测二级结构的RNA进行敏感且无标签的生物传感

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摘要

A novel biosensing approach for the label-free detection of nucleic acid sequences of short and large lengths has been implemented, with special emphasis on targeting RNA sequences with secondary structures. The approach is based on selecting 8-aminoadenine-modified parallel-stranded DNA tail-clamps as affinity bioreceptors. These receptors have the ability of creating a stable triplex-stranded helix at neutral pH upon hybridization with the nucleic acid target. A surface plasmon resonance biosensor has been used for the detection. With this strategy, we have detected short DNA sequences (32-mer) and purified RNA (103-mer) at the femtomol level in a few minutes in an easy and level-free way. This approach is particularly suitable for the detection of RNA molecules with predicted secondary structures, reaching a limit of detection of 50 fmol without any label or amplification steps. Our methodology has shown a marked enhancement for the detection (18% for short DNA and 54% for RNA), when compared with the conventional duplex approach, highlighting the large difficulty of the duplex approach to detect nucleic acid sequences, especially those exhibiting stable secondary structures. We believe that our strategy could be of great interest to the RNA field.
机译:已经实现了一种新颖的生物传感方法,用于短和大长度的核酸序列的无标记检测,特别是针对具有二级结构的RNA序列。该方法基于选择8-氨基腺嘌呤修饰的平行链DNA尾夹作为亲和力生物受体。这些受体具有在与核酸靶杂交后在中性pH下产生稳定的三链螺旋的能力。表面等离子体激元共振生物传感器已经用于检测。通过这种策略,我们可以在数分钟内以简便,无水平的方式检测到飞摩尔水平的短DNA序列(32-mer)和纯化的RNA(103-mer)。这种方法特别适用于检测具有预测二级结构的RNA分子,无需任何标记或扩增步骤即可达到50 µfmol的检测限。与传统的双链方法相比,我们的方法显示出显着的检测增强(短DNA的18%和RNA的54%),突显了双链方法检测核酸序列的难度很大,尤其是那些表现出稳定二级序列的核酸序列结构。我们认为,我们的策略可能对RNA领域非常重要。

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