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首页> 外文期刊>Langmuir: The ACS Journal of Surfaces and Colloids >Ordered self-assembled locked nucleic acid (LNA) structures on gold(111) surface with enhanced single base mismatch recognition capability
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Ordered self-assembled locked nucleic acid (LNA) structures on gold(111) surface with enhanced single base mismatch recognition capability

机译:具有增强的单碱基错配识别能力的金(111)表面上的有序自组装锁定核酸(LNA)结构

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摘要

Locked nucleic acid (LNA) is a conformationally restricted nucleic acid analogue, which is potentially a better alternative than DNA for application in the nucleic acid based biosensor technologies, due to its efficient and sequence-specific DNA/RNA detection capability and lack of molecule-surface interaction on solid surfaces, compared to DNA. We report, for the first time, a straightforward way (based on simple immersion method) of generating an ordered self-assembled LNA monolayer, which is bioactive, onto a gold(111) surface. This layer is capable of giving rise to a stronger DNA recognition signal (4-4.5 times) than its DNA counterpart, and importantly, it can differentiate between a fully complementary DNA target and that having a single base mismatch, where the mismatch discrimination ratio is almost two times compared to the ratio relevant in case of DNA-based detection. We have presented high-resolution atomic force microscopy (AFM) topographs of the well-defined one-dimensional LNA molecular ordering (few hundred nanometers long) and of the two-dimensional ordered assembly formed over a large area (7 μm × 7 μm) due to parallel positioning of the one-dimensional ordered arrangements. The effects of different parameters such as LNA concentration and incubation time on LNA self-assembly have been investigated. Further, reflection absorption infrared (RAIR) spectroscopy has been applied to obtain information about the orientation of the surface-immobilized LNA molecules for the first time. It has been found that the LNA molecules undergo an orientational transition from the "lying down" to the "upright" configuration in a time scale of few hours.
机译:锁定核酸(LNA)是一种受构象限制的核酸类似物,由于其高效且具有序列特异性的DNA / RNA检测能力以及缺乏分子识别技术,因此它可能比DNA更好地替代基于核酸的生物传感器技术。与DNA相比,固体表面上的表面相互作用。我们首次报告了一种直接的方法(基于简单的浸入方法),该方法在金(111)表面上生成具有生物活性的有序自组装LNA单层。该层能够产生比其DNA对应物更强的DNA识别信号(4-4.5倍),重要的是,它可以区分完全互补的DNA靶标和具有单个碱基错配的靶标,其中错配识别率是几乎是基于DNA的检测比例的两倍。我们提供了高分辨率的原子力显微镜(AFM)形貌图,该图的轮廓分明,是一维LNA分子序(长几百纳米),并且是在大面积(7μm×7μm)上形成的二维有序组件由于一维有序排列的平行放置。研究了不同参数(例如LNA浓度和孵育时间)对LNA自组装的影响。此外,反射吸收红外(RAIR)光谱已被首次用于获得有关表面固定LNA分子取向的信息。已经发现,LNA分子在几个小时的时间尺度上经历从“躺下”到“竖立”构型的定向转变。

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