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炔基修饰的 DNA 功能化合金 Au/Ag 纳米球用于比率型表面增强拉曼散射成像分析活细胞内内切酶活性

Alkyne-DNA-Functionalized Alloyed Au/Ag Nanospheres for Ratiometric Surface-Enhanced Raman Scattering Imaging Assay of Endonuclease Activity in Live Cells.

机构信息

State Key Laboratory of Chemo/Bio-Sensing and Chemometrics, College of Chemistry and Chemical Engineering, Institute of Chemical Biology and Nanomedicine , Hunan University , Changsha 410082 , China.

Department of Chemistry , University of California-Riverside , Riverside , California 92521 , United States.

出版信息

Anal Chem. 2018 Mar 20;90(6):3898-3905. doi: 10.1021/acs.analchem.7b04735. Epub 2018 Mar 9.

Abstract

A novel ratiometric surface-enhanced Raman scattering (SERS) nanosensor has been developed to probe the activity of endonuclease under in vitro and in living cells conditions. The optimized alloyed Au/Ag nanoparticles (NPs) were synthesized as the SERS substrate, which combined the superior properties of both pure Au and pure Ag nanoparticles: they exhibit excellent plasmonic property with high chemical stability and low cytotoxicity. They were then employed for quantitative detection of endonuclease through functionalization with single-stranded DNA (ssDNA) carrying 3-[4-(phenylethynyl)benzylthio]propanoic acid (PEB) as endonuclease-responsive SERS signaling molecule and 4-thiophenylacetylene (TPA) as the internal standard SERS signaling molecule. In the presence of endonuclease, the ssDNA was cleaved, releasing PEB molecules from the particle surface and decreasing the SERS signal at 2215 cm from PEB. Since the SERS signal at 1983 cm from alkynyl TPA remained the same, quantitative detection of endonuclease was achieved, based on the ratiometric peak intensity of I/ I, with a detection limit as low as 0.056 unit/mL. A highly biocompatible and antijamming ratiometric SERS sensor was established by combining the alloyed Au/AgNPs with two unique alkynes molecules with Raman signals in the cellular silent region. The ratiometric sensor was successfully employed to detect intracellular endonuclease activity as well as endonuclease in living cells for the first time.

摘要

一种新型的比率型表面增强拉曼散射(SERS)纳米传感器已被开发出来,用于在体外和活细胞条件下探测内切核酸酶的活性。优化的合金 Au/Ag 纳米粒子(NPs)被合成作为 SERS 基底,它结合了纯 Au 和纯 Ag 纳米粒子的优越性能:它们具有优异的等离子体特性,具有高化学稳定性和低细胞毒性。然后,它们通过用携带 3-[4-(苯乙炔基)苄硫基]丙酸(PEB)的单链 DNA(ssDNA)功能化,用作内切核酸酶响应的 SERS 信号分子,并用 4-巯基苯乙炔(TPA)作为内部标准 SERS 信号分子,用于定量检测内切核酸酶。在存在内切核酸酶的情况下,ssDNA 被切割,从粒子表面释放出 PEB 分子,从而降低了来自 PEB 的 2215cm 的 SERS 信号。由于来自炔基 TPA 的 1983cm 的 SERS 信号保持不变,因此可以基于 I/ I 的比率峰强度进行定量检测,检测限低至 0.056 单位/mL。通过将合金 Au/AgNPs 与具有在细胞静默区中具有拉曼信号的两个独特炔烃分子结合,建立了一种高度生物相容性和抗干扰的比率 SERS 传感器。该比率传感器成功地用于首次检测细胞内内切核酸酶活性和活细胞中的内切核酸酶。

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