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DNAzyme 扩增级联催化发夹组装纳米系统用于活细胞中敏感的 microRNA 成像。

DNAzyme-Amplified Cascade Catalytic Hairpin Assembly Nanosystem for Sensitive MicroRNA Imaging in Living Cells.

机构信息

Guangdong Provincial Key Laboratory of Sensing Technology and Biomedical Instrument, School of Biomedical Engineering, Shenzhen Campus of Sun Yat-Sen University, Sun Yat-Sen University, Shenzhen 518107, China.

School of Chemistry, Sun Yat-Sen University, Guangzhou 510275, China.

出版信息

Anal Chem. 2023 Aug 8;95(31):11793-11799. doi: 10.1021/acs.analchem.3c02071. Epub 2023 Jul 4.

DOI:10.1021/acs.analchem.3c02071
PMID:37402285
Abstract

Sensitive imaging of microRNAs (miRNAs) in living cells is significant for accurate cancer clinical diagnosis and prognosis research studies, but it is challenged by inefficient intracellular delivery, instability of nucleic acid probes, and limited amplification efficiency. Herein, we engineered a DNAzyme-amplified cascade catalytic hairpin assembly (CHA)-based nanosystem (DCC) that overcomes these challenges and improves the imaging sensitivity. This enzyme-free amplification nanosystem is based on the sequential activation of DNAzyme amplification and CHA. MnO nanosheets were used as nanocarriers for the delivery of nucleic acid probes, which can resist the degradation by nucleases and supply Mn for the DNAzyme reaction. After entering into living cells, the MnO nanosheets can be decomposed by intracellular glutathione (GSH) and release the loaded nucleic acid probes. In the presence of target miRNA, the locking strand (L) was hybridized with target miRNA, and the DNAzyme was released, which then cleaved the substrate hairpin (H). This cleavage reaction resulted in the formation of a trigger sequence (TS) that can activate CHA and recover the fluorescence readout. Meanwhile, the DNAzyme was released from the cleaved H and bound to other H for new rounds of DNAzyme-based amplification. The TS was also released from CHA and involved in the new cycle of CHA. By this DCC nanosystem, low-abundance target miRNA can activate many DNAzyme and generate numerous TS for CHA, resulting in sensitive and selective analysis of miRNAs with a limit of detection of 5.4 pM, which is 18-fold lower than that of the traditional CHA system. This stable, sensitive, and selective nanosystem holds great potential for miRNA analysis, clinical diagnosis, and other related biomedical applications.

摘要

在活细胞中对 microRNAs (miRNAs) 进行敏感成像对于准确的癌症临床诊断和预后研究非常重要,但这受到核酸探针内效率低、核酸探针不稳定性和有限的扩增效率的挑战。在此,我们设计了一种基于 DNAzyme 放大级联催化发夹组装 (CHA) 的纳米系统 (DCC),克服了这些挑战并提高了成像灵敏度。这种无酶扩增纳米系统基于 DNAzyme 扩增和 CHA 的顺序激活。MnO 纳米片被用作核酸探针的递送纳米载体,其可以抵抗核酸酶的降解并为 DNAzyme 反应提供 Mn。进入活细胞后,MnO 纳米片可以被细胞内的谷胱甘肽 (GSH) 分解并释放负载的核酸探针。在存在靶 miRNA 的情况下,锁定链 (L) 与靶 miRNA 杂交,释放 DNAzyme,然后切割底物发夹 (H)。该切割反应导致形成触发序列 (TS),其可以激活 CHA 并恢复荧光读出。同时,DNAzyme 从被切割的 H 中释放出来并与其他 H 结合以进行新的一轮基于 DNAzyme 的扩增。TS 也从 CHA 中释放出来并参与 CHA 的新循环。通过这种 DCC 纳米系统,低丰度靶 miRNA 可以激活许多 DNAzyme 并生成许多用于 CHA 的 TS,从而实现对 miRNA 的灵敏和选择性分析,检测限低至 5.4 pM,比传统 CHA 系统低 18 倍。这种稳定、灵敏和选择性的纳米系统在 miRNA 分析、临床诊断和其他相关生物医学应用中具有很大的潜力。

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