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在金(111)表面有序排列的自组装锁定核酸(LNA)结构,具有增强的单碱基错配识别能力。

Ordered self-assembled locked nucleic acid (LNA) structures on gold(111) surface with enhanced single base mismatch recognition capability.

机构信息

Department of Biological Chemistry, Indian Association for the Cultivation of Science, Jadavpur, Kolkata, India.

出版信息

Langmuir. 2012 Mar 6;28(9):4325-33. doi: 10.1021/la204026j. Epub 2012 Feb 23.

Abstract

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.

摘要

锁核酸(LNA)是一种构象受限的核酸类似物,与 DNA 相比,它具有高效、序列特异性的 DNA/RNA 检测能力,并且在固体表面上缺乏分子-表面相互作用,因此有可能成为核酸基生物传感器技术的更好选择。我们首次报道了一种简单的方法(基于简单的浸渍法),可在金(111)表面生成有序的自组装 LNA 单层,该单层具有生物活性。与 DNA 相比,这种单层能够产生更强的 DNA 识别信号(增强 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,其中错配的区分率几乎是基于 DNA 检测的相关比率的两倍。我们已经展示了高分辨率原子力显微镜(AFM)的形貌图,这些形貌图显示了一维 LNA 分子有序排列(几百纳米长)和二维有序组装(由于一维有序排列的平行定位,面积达 7 μm×7 μm)。研究了不同参数(如 LNA 浓度和孵育时间)对 LNA 自组装的影响。此外,首次应用反射吸收红外(RAIR)光谱获得了关于表面固定 LNA 分子取向的信息。结果发现,LNA 分子在数小时的时间内经历了从“躺下”到“直立”构型的取向转变。

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