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通过新的分子转子对细胞内粘度进行成像,该分子转子适用于荧光寿命相分析。

Imaging intracellular viscosity by a new molecular rotor suitable for phasor analysis of fluorescence lifetime.

机构信息

NEST, Scuola Normale Superiore and Istituto Nanoscienze, CNR, Pisa, Italy.

出版信息

Anal Bioanal Chem. 2013 Jul;405(19):6223-33. doi: 10.1007/s00216-013-7084-x. Epub 2013 Jun 19.

Abstract

The arsenal of fluorescent probes tailored to functional imaging of cells is rapidly growing and benefits from recent developments in imaging strategies. Here, we present a new molecular rotor, which displays strong absorption in the green region of the spectrum, very little solvatochromism, and strong emission sensitivity to local viscosity. The emission increase is paralleled by an increase in emission lifetime. Owing to its concentration-independent nature, fluorescence lifetime is particularly suitable to image environmental properties, such as viscosity, at the intracellular level. Accordingly, we demonstrate that intracellular viscosity measurements can be efficiently carried out by lifetime imaging with our probe and phasor analysis, an efficient method for measuring lifetime-related properties (e.g., bionalyte concentration or local physicochemical features) in living cells. Notably, we show that it is possible to monitor the partition of our probe into different intracellular regions/organelles and to follow mitochondrial de-energization upon oxidative stress.

摘要

针对细胞功能成像而定制的荧光探针库正在迅速发展,并受益于成像策略的最新进展。在这里,我们提出了一种新的分子转子,它在光谱的绿色区域显示出很强的吸收,很少有溶剂变色,并且对局部粘度具有很强的发射灵敏度。发射的增加伴随着发射寿命的增加。由于其浓度无关的性质,荧光寿命特别适合在细胞内水平上成像环境特性,例如粘度。因此,我们证明可以通过使用我们的探针和相分析进行寿命成像来有效地进行细胞内粘度测量,相分析是一种测量活细胞中与寿命相关的特性(例如双离子浓度或局部物理化学特征)的有效方法。值得注意的是,我们表明可以监测我们的探针分配到不同的细胞内区域/细胞器中,并在氧化应激时跟踪线粒体去极化。

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