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面对面组装金纳米立方体策略:用于细胞内 miRNA 的 SERS-荧光双信号检测的宽热点区域的诱导产生。

Face-to-face Assembly Strategy of Au Nanocubes: Induced Generation of Broad Hotspot Regions for SERS-Fluorescence Dual-Signal Detection of Intracellular miRNAs.

机构信息

Center of Clinical Laboratory Medicine, Zhongda Hospital, Medical School of Southeast University, Nanjing, Jiangsu 210009, China.

Jiangsu Key Laboratory of New Drug Research and Clinical Pharmacy, School of Pharmacy, Xuzhou Medical University, Xuzhou 221004, China.

出版信息

Anal Chem. 2024 Jun 4;96(22):8922-8931. doi: 10.1021/acs.analchem.3c05743. Epub 2024 May 17.

DOI:10.1021/acs.analchem.3c05743
PMID:38758935
Abstract

While designing anisotropic noble metal nanoparticles (NPs) can enhance the signal intensity of Raman dyes, more sensitive surface-enhanced Raman scattering (SERS) probes can be designed by oriented self-assembly of noble metal nanomaterials into dimers or higher-order nanoclusters. In this study, we engineered a self-assembly strategy in living cells for real-time fluorescence and SERS dual-channel detection of intracellular microRNAs (miRNAs), using Mg-dependent 8-17E DNAzyme sequences as the driving motors, gold nanocubes (AuNCs) as the driver components, and three-branched double-stranded DNA as the linking tool. The assembly selects adenine in DNA as a reporter molecule, simplifying the labeling process of Raman reporter molecules and reducing the synthesis process. In addition, adenine is stably distributed between the faces of AuNCs and the wide hotspot region gives good reproducibility of the adenine SERS signal. In this strategy, the SERS channel was consistently stable and more sensitive compared to the fluorescence channel. Among them, the detection limit of the SERS channel was 2.1 pM and the coefficient of variation was 1.26% in the in vitro liquid phase and 1.49% in MCF-7 cells. The strategy successfully achieved accurate tracking and quantification of miRNA-21 in cancer cells, showing good reproducibility in complex samples as well as cells. The reported strategy provides ideas for exploring intracellular specific triggering of nanoparticles for precise control of self-assembly.

摘要

在设计各向异性贵金属纳米粒子(NPs)时,可以增强拉曼染料的信号强度,通过将贵金属纳米材料定向自组装成二聚体或更高阶的纳米簇,可以设计出更灵敏的表面增强拉曼散射(SERS)探针。在这项研究中,我们设计了一种在活细胞内进行的自组装策略,用于实时荧光和 SERS 双通道检测细胞内 microRNAs(miRNAs),使用 Mg 依赖性 8-17E DNA 酶序列作为驱动马达,金纳米立方体(AuNCs)作为驱动组件,三臂双链 DNA 作为连接工具。该组装选择 DNA 中的腺嘌呤作为报告分子,简化了拉曼报告分子的标记过程,减少了合成过程。此外,腺嘌呤稳定地分布在 AuNCs 的表面之间,并且宽热点区域使腺嘌呤的 SERS 信号具有良好的重现性。在该策略中,SERS 通道与荧光通道相比始终保持稳定且更灵敏。其中,在体外液相和 MCF-7 细胞中,SERS 通道的检测限分别为 2.1 pM 和 1.49%,其变异系数分别为 1.26%和 1.49%。该策略成功实现了对癌细胞中 miRNA-21 的准确跟踪和定量,在复杂样本和细胞中也表现出良好的重现性。该报告的策略为探索用于精确控制自组装的纳米颗粒的细胞内特定触发提供了思路。

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