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一种近红外遥控上转换纳米粒子:用于活细胞染料标记的改进工具。

A NIR-remote controlled upconverting nanoparticle: an improved tool for living cell dye-labeling.

作者信息

Zheng Bin, Gong Xiaoqun, Wang Hanjie, Wang Sheng, Wang Huiquan, Li Wei, Tan Jian, Chang Jin

机构信息

School of Life Sciences, Tianjin University, Collaborative Innovation Center of Chemical Science and Engineering (Tianjin), 92 Weijin Road, Nankai District, Tianjin 300072, People's Republic of China.

出版信息

Nanotechnology. 2015 Oct 23;26(42):425102. doi: 10.1088/0957-4484/26/42/425102. Epub 2015 Sep 30.

Abstract

In living cells, due to the selective permeability and complicated cellular environment, the uptake efficiency and fluorescence decay of organic dyes during dye-labeling may be influenced, which may eventually result in poor fluorescent imaging. In this work, a protocol of UCNs@mSiO2-(FA and Azo) core-shell nanocarriers was designed and prepared successfully. The core-shell nanocarriers were assembled from two parts, including a mesoporous silica shell surface modified by folate (FA) and azobenzene (Azo), and an upconverting nanocrystal (UCN) core. The mesoporous silica shell is used for loading organic dyes and conjugating folate which helps to enhance the cellular uptake of nanocarriers. The UCN core works as a transducer to convert near infrared (NIR) light to local UV and visible light to activate a back-and-forth wagging motion of azobenzene molecules on the surface, while the azobenzene acts as a molecular impeller for propelling the release of organic dyes. The nanocarriers of loading organic dyes can maintain the stability of the fluorescent imaging effect better than free organic dyes. The experimental results show that with the help of the nanoparticle, cell uptake efficiency of the model dyes of rhodamine and 4', 6-diamidino-2-phenylindole (DAPI) was significantly improved. The release of dyes can only be triggered by NIR light exposure and their quantity is highly dependent on the duration of NIR light exposure, thus realizing NIR-regulated dye release spatiotemporally. Our work may open a novel avenue for precisely controlling UCN-based living cell imaging in biotechnology and diagnostics, as well as studying cell dynamics, cell-cell interactions, and tissue morphogenesis.

摘要

在活细胞中,由于选择性通透性和复杂的细胞环境,染料标记过程中有机染料的摄取效率和荧光衰减可能会受到影响,最终可能导致荧光成像效果不佳。在这项工作中,成功设计并制备了一种UCNs@mSiO2-(FA和Azo)核壳纳米载体方案。核壳纳米载体由两部分组装而成,包括通过叶酸(FA)和偶氮苯(Azo)修饰的介孔二氧化硅壳表面,以及上转换纳米晶体(UCN)核。介孔二氧化硅壳用于负载有机染料并偶联叶酸,这有助于增强纳米载体的细胞摄取。UCN核作为换能器,将近红外(NIR)光转换为局部紫外光和可见光,以激活表面偶氮苯分子的来回摆动运动,而偶氮苯则作为分子叶轮推动有机染料的释放。负载有机染料的纳米载体比游离有机染料能更好地保持荧光成像效果的稳定性。实验结果表明,在纳米颗粒的帮助下,罗丹明和4',6-二脒基-2-苯基吲哚(DAPI)等模型染料的细胞摄取效率显著提高。染料的释放只能通过近红外光照射触发,其释放量高度依赖于近红外光照射的持续时间,从而实现近红外光时空调控的染料释放。我们的工作可能为生物技术和诊断中基于UCN的活细胞成像的精确控制,以及研究细胞动力学、细胞间相互作用和组织形态发生开辟一条新途径。

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