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Specific binding and internalization: an investigation of fluorescent aptamer-gold nanoclusters and cells with fluorescence lifetime imaging microscopy

机译:具体的绑定和内化:一个调查荧光aptamer-gold制备和细胞荧光寿命成像显微镜

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摘要

Fluorescent gold nanoclusters show promising properties for biological applications. We biofunctionalized fluorescent 11-mercaptoundecanoic-acid stabilized gold nanoclusters (AuNCs) with an aptamer to target the interleukin-6-receptor expressed on BaF3 cells specifically. Although the fluorescence emission of the AuNCs (535 nm) is in the same wavelength region as the autofluorescence of the cell, we are able to distinguish between nanoclusters and cells using the fluorescence decay time, which is much longer for the AuNCs (100 ns) than for the autofluorescence. After a first short incubation period we detected AuNCs specifically bound to the cell membrane by using two fluorescence lifetime imaging microscopy (FLIM) methods: gated and direct FLIM. After a second incubation period the previously bound AuNCs are internalized by the cells, as could be resolved solely by the direct FLIM. This proves the superior sensitivity of this method compared to gated FLIM. We find that the optical properties of AuNCs do not change upon binding to the cells, but exhibit a change when internalized into the cells, induced by an interaction between the AuNCs and cells.
机译:荧光金纳米束显示有前途生物应用程序属性。biofunctionalized荧光11-mercaptoundecanoic-acid稳定黄金制备(AuNCs)与一个适配子目标BaF3 interleukin-6-receptor表示细胞特别。发射的AuNCs(535海里)是相同的自发荧光的波长区域细胞,我们能够区分使用荧光发光机制和细胞衰减时间,AuNCs更长(100 ns)比自体荧光。首先我们发现AuNCs短潜伏期特别是绑定到细胞膜通过使用两个荧光寿命成像显微镜(这部电影)方法:封闭的和直接的这部电影。第二个潜伏期以前绑定AuNCs内化的细胞,可以解决完全由直接的这部电影。这种方法相比的优越的敏感性封闭的这部电影。AuNCs不改变在绑定的属性细胞,但是当内化而改变进入细胞,诱导之间的交互AuNCs和细胞。

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