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Sensitive Detection of Nucleic Acids with Rolling Circle Amplification and Surface-Enhanced Raman Scattering Spectroscopy

机译:滚圆扩增和表面增强拉曼散射光谱法灵敏检测核酸

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摘要

Detection of specific DNA sequences is important to molecular biology research and clinical diagnostics. To improve the sensitivity of surface-enhanced Raman scattering spectroscopy (SERS), a variety of signal amplification methods has been developed, including Raman-active-dye, polymerase chain reaction (PCR) technology, molecular beacon, SERS-active substrates, and SERS-tag. However, the combination of rolling circle amplification (RCA) with SERS for nucleic acid detection has not been reported. Herein, we describe a new approach for nucleic acid detection by the combination of RCA reaction with SERS. Because of the binding of abundance repeated sequences of RCA products with gold nanoparticle (Au NP) and Rox-modified detection probes, SERS signal is significantly amplified and the detection limit of 10.0 pM might be achieved. The sensitivity of RCA-based SERS has increased by as much as 3 orders of magnitude as compared to PCR-based SERS and is also comparable with or even exceeds that of both RCA-based electrochemical and RCA-based fluorescent methods. This RCA-based SERS might discriminate perfect matched target DNA from 1-base mismatched DNA with high selectivity. The high sensitivity and selectivity of RCA-based SERS makes it a potential tool for early diagnosis of gene-related disease and also offers a great promise for multiplexed assays with DNA microarrays.
机译:特定DNA序列的检测对于分子生物学研究和临床诊断很重要。为了提高表面增强拉曼散射光谱(SERS)的灵敏度,已经开发了多种信号放大方法,包括拉曼活性染料,聚合酶链反应(PCR)技术,分子信标,SERS活性底物和SERS -标签。然而,尚未报道滚环扩增(RCA)与SERS结合用于核酸检测。在本文中,我们描述了一种通过RCA反应与SERS结合进行核酸检测的新方法。由于RCA产物的大量重复序列与金纳米粒子(Au NP)和Rox修饰的检测探针结合,SERS信号得到了显着放大,检测限为10.0 pM。与基于PCR的SERS相比,基于RCA的SERS的灵敏度提高了多达3个数量级,并且与基于RCA的电化学方法和基于RCA的荧光方法相比,甚至更高甚至更高。这种基于RCA的SERS可以高选择性地将完全匹配的靶DNA与1个碱基错配的DNA区分开。基于RCA的SERS的高灵敏度和选择性使其成为基因相关疾病早期诊断的潜在工具,也为使用DNA微阵列进行多重检测提供了广阔的前景。

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