Dimerizing DNA-AgNCs via a C–Ag+–C structure for fluorescence sensing with dual-output signals†

IF 4.2 2区化学 Q2 CHEMISTRY, MULTIDISCIPLINARY

Chemical Communications Pub Date : 2025-01-14 DOI:10.1039/d4cc06687a

Shuai Chen , Wenjie Hu , Yuqi Cheng , Zhiwei Yin , Jiaxiang Xiao , Changwen Li , Haihong Zhao , Qian Dong , Zhuo Chen

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Abstract

The unique insertion capability of Ag⁺ into cytosine–cytosine (C–Ag⁺–C) mismatch-base pairs enables precise fabrication of DNA-trapped silver nanoclusters (DNA-AgNCs) through varying the DNA sequences, thereby offering precise assembly of DNA-AgNCs and demonstrating great fluorescence applications. However, most of the DNA-AgNC-based fluorescence sensors have a single output signal. Herein, we developed a dimerized DNA-AgNC system through C–Ag⁺–C connection at the 3′-end of a designed DNA. The formation and crack-up of C–Ag⁺–C endows DNA-AgNCs with the ability to identify Ag⁺ and cysteine (Cys) with dual-output signals, changed fluorescence intensity (FI) and wavelength-shift in NIR emission around 815 nm via photoinduced electron transfer (PET), respectively. Superior linearity of FI for Cys and Ag⁺ concentrations was demonstrated. Meanwhile, the practical utility of this platform was also successfully verified in milk and lake water.

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通过C-Ag+ c结构对dna - agnc进行二聚化，用于双输出信号的荧光传感

Ag+独特的插入胞嘧啶-胞嘧啶（C-Ag+-C）错配碱基对的能力，使得通过改变DNA序列来精确制造DNA捕获银纳米团簇（DNA- agnc），从而提供DNA- agnc的精确组装，并展示了巨大的荧光应用。然而，大多数基于dna - agncs的荧光传感器具有单一输出信号。在此，我们通过设计的DNA的3'端C-Ag+-C连接开发了二聚化DNA- agnc系统。C-Ag+-C的形成和裂解使dna - agnc能够通过双输出信号识别Ag+和半胱氨酸（Cys），通过光诱导电子转移（PET）分别改变荧光强度（FI）和近红外发射波长移（约815 nm）。结果表明，FI对Cys和Ag+浓度具有良好的线性关系。同时，在牛奶和湖水中也成功验证了该平台的实用性。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

Chemical Communications 化学-化学综合

CiteScore

8.60

自引率

4.10%

发文量

2705

审稿时长

1.4 months

期刊介绍： ChemComm (Chemical Communications) is renowned as the fastest publisher of articles providing information on new avenues of research, drawn from all the world''s major areas of chemical research.