双分子荧光互补
荧光蛋白
荧光
绿色荧光蛋白
体内
蛋白质-蛋白质相互作用
互补
生物
生物物理学
合理设计
黄色荧光蛋白
临床前影像学
细胞生物学
蛋白质片段互补分析
蛋白质工程
荧光素酶
生物化学
转染
遗传学
基因
突变体
酶
量子力学
物理
作者
Grigory S. Filonov,Vladislav V. Verkhusha
出处
期刊:Chemistry & Biology
[Elsevier BV]
日期:2013-07-25
卷期号:20 (8): 1078-1086
被引量:95
标识
DOI:10.1016/j.chembiol.2013.06.009
摘要
Studies of protein-protein interactions deep in organs and in whole mammals have been hindered by a lack of genetically encoded fluorescent probes in near-infrared region for which mammalian tissues are the most transparent. We have used a near-infrared fluorescent protein iRFP engineered from a bacterial phytochrome as the template to develop an in vivo split fluorescence complementation probe. The domain architecture-based rational design resulted in an iSplit reporter with the spectra optimal for whole-body imaging, high photostability, and high complementation contrast, which compares favorably to that of other available split fluorescent protein-based probes. Successful visualization of interaction of two known protein partners in a living mouse model suggests iSplit as the probe of choice for noninvasive detection of protein-protein interactions in vivo, whereas its fast intracellular degradation enables time-resolved monitoring of repetitive binding events.
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