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Characterization of Flavin-Based Fluorescent Proteins: An Emerging Class of Fluorescent Reporters

机译:基于黄素的荧光蛋白的表征:一类新兴的荧光报道分子

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摘要

Fluorescent reporter proteins based on flavin-binding photosensors were recently developed as a new class of genetically encoded probes characterized by small size and oxygen-independent maturation of fluorescence. Flavin-based fluorescent proteins (FbFPs) address two major limitations associated with existing fluorescent reporters derived from the green fluorescent protein (GFP)–namely, the overall large size and oxygen-dependent maturation of fluorescence of GFP. However, FbFPs are at a nascent stage of development and have been utilized in only a handful of biological studies. Importantly, a full understanding of the performance and properties of FbFPs as a practical set of biological probes is lacking. In this work, we extensively characterize three FbFPs isolated from Pseudomonas putida, Bacillus subtilis, and Arabidopsis thaliana, using in vitro studies to assess probe brightness, oligomeric state, maturation time, fraction of fluorescent holoprotein, pH tolerance, redox sensitivity, and thermal stability. Furthermore, we validate FbFPs as stable molecular tags using in vivo studies by constructing a series of FbFP-based transcriptional constructs to probe promoter activity in Escherichia coli. Overall, FbFPs show key advantages as broad-spectrum biological reporters including robust pH tolerance (4–11), thermal stability (up to 60°C), and rapid maturation of fluorescence (<3 min.). In addition, the FbFP derived from Arabidopsis thaliana (iLOV) emerged as a stable and nonperturbative reporter of promoter activity in Escherichia coli. Our results demonstrate that FbFP-based reporters have the potential to address key limitations associated with the use of GFP, such as pH-sensitive fluorescence and slow kinetics of fluorescence maturation (10–40 minutes for half maximal fluorescence recovery). From this view, FbFPs represent a useful new addition to the fluorescent reporter protein palette, and our results constitute an important framework to enable researchers to implement and further engineer improved FbFP-based reporters with enhanced brightness and tighter flavin binding, which will maximize their potential benefits.
机译:最近,基于黄素结合型光电传感器的荧光报告蛋白被开发为一类新的遗传编码探针,其特征是小尺寸和不依赖氧的荧光成熟。基于黄素的荧光蛋白(FbFP)解决了与绿色荧光蛋白(GFP)衍生的现有荧光报告基因相关的两个主要限制,即GFP荧光的整体大小和氧依赖性成熟。但是,FbFPs尚处于发展初期,仅用于少数生物学研究中。重要的是,缺乏对FbFPs作为一组实用的生物探针的性能和特性的全面了解。在这项工作中,我们使用体外研究评估探针的亮度,寡聚状态,成熟时间,荧光全卤化分数,pH耐受性,氧化还原敏感性和热稳定性,广泛表征了从恶臭假单胞菌,枯草芽孢杆菌和拟南芥中分离出的三种FbFP。 。此外,我们通过构建一系列基于FbFP的转录构建体来探测大肠杆菌中的启动子活性,利用体内研究验证了FbFPs作为稳定的分子标签。总体而言,FbFP作为广谱生物学报道分子显示出关键优势,包括强大的pH耐受性(4-11),热稳定性(最高60°C)和荧光的快速成熟(<3分钟)。另外,源自拟南芥的FbFP(iLOV)作为大肠杆菌中启动子活性的稳定且无干扰的报告基因出现。我们的结果表明,基于FbFP的报告基因有可能解决与GFP使用相关的关键局限性,例如pH敏感的荧光和缓慢的荧光成熟动力学(最大荧光恢复一半需要10-40分钟)。从这个角度来看,FbFPs代表了荧光报告基因蛋白调色板的有用的新成员,我们的结果构成了一个重要的框架,使研究人员能够实施和进一步设计改良的基于FbFP的报告基因,并具有更高的亮度和更强的黄素结合力,这将最大限度地发挥其潜力。好处。

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