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首页> 外文期刊>ACS Chemical Biology >Indole-based Cyanine as a Nuclear RNA-Selective Two-Photon Fluorescent Probe for Live Cell Imaging
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Indole-based Cyanine as a Nuclear RNA-Selective Two-Photon Fluorescent Probe for Live Cell Imaging

机译:基于吲哚的花菁作为活细胞成像的核RNA选择性双光子荧光探针。

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摘要

We have demonstrated that the subcellular targeting properties of the indole-based cyanines can be tuned by the functional substituent attached onto the indole moiety in which the first example of a highly RNA-selective and two-photon active fluorescent light-up probe for high contrast and brightness TPEF images of rRNA in the nucleolus of live cells has been developed. It is important to find that this cyanine binds much stronger toward RNA than DNA in a buffer solution as well as selectively stains and targets to rRNA in the nucleolus. Remarkably, the TPEF brightness (phi sigma(max)) is dramatically increased with 11-fold enhancement in the presence of rRNA, leading to the record high phi sigma(max) of 228 GM for RNA. This probe not only shows good biocompatibility and superior photostability but also offers general applicability to various live cell lines including HeLa, HepG2, MCF-7, and KB cells and excellent counterstaining compatibility with commercially available DNA or protein trackers.
机译:我们已经证明,吲哚类花菁的亚细胞靶向特性可以通过吲哚部分上连接的功能性取代基进行调节,其中第一个高RNA选择性和双光子活性荧光发光探针的高对比度实例已经开发了活细胞核仁中rRNA的高亮度TPEF图像。重要的是要发现,这种花青素与RNA的结合要比缓冲溶液中的DNA强得多,并且可以选择性地染色和靶向核仁中的rRNA。值得注意的是,在存在rRNA的情况下,TPEF亮度(phi sigma(max))显着提高了11倍,导致RNA达到228 GM的创纪录高phi sigma(max)。该探针不仅显示出良好的生物相容性和优异的光稳定性,而且还广泛适用于包括HeLa,HepG2,MCF-7和KB细胞在内的各种活细胞系,并与市售DNA或蛋白质示踪剂具有出色的复染相容性。

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