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Modeling and Experimental Validation of Large Scale Fluorescence Sensor Networks

机译:大规模荧光传感器网络的建模与实验验证

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Fluorescence microscopy is by far the dominant assay used to measure molecular scale interactions in a wide range of disciplines including biochemistry, biophysics, bioengineering, biomedical imaging and clinical diagnostics. However, the technique can probe only a small number of molecular interactions with previous attempts at detecting more than 11 fluorophores simultaneously resulting in barcodes that are too big for in vivo analysis, expensive and involve time-consuming detection schemes. Here, we create DNA self-assembled Resonance Energy Transfer networks that generate a unique time-resolved fluorescence signature when probed by a series of light pulses. An experimentally informed theoretical model predicts that networks containing up to 125 fluorophores may be distinguished from other extremely similar networks. Through the largest experimental survey of RET networks, we demonstrate that minor changes made to the RET network result in a unique, experimentally resolvable optical signature. We show that we can generate over 300 unique signatures using only 3 fluorophores. Furthermore, from 1296 time-resolved fluorescence signatures, we show that the optical signatures are reproducible 99.48% of the time. The ability to simultaneously detect multiple biological entities, the high spatial information density and the high repeatability of the synthetic RET networks will potentially find use in many biological and clinical applications.
机译:荧光显微镜是迄今为止的主要测定,用于测量包括生物化学,生物物理学,生物工程,生物医学成像和临床诊断的各种学科中的分子尺度相互作用。然而,该技术只能探测少量的分子相互作用与先前的尝试检测超过11个荧光团,同时导致用于体内分析的条形码太大,昂贵并涉及耗时的检测方案。在这里,我们创建DNA自组装的共振能量转移网络,当通过一系列光脉冲探测时,产生独特的时间分辨荧光签名。实验上通知的理论模型预测,包含多达125荧光团的网络可以与其他极其相似的网络区分开。通过对RET网络的最大实验调查,我们证明对RET网络的微小变化导致独特的实验可解析的光学签名。我们表明我们只能使用3种荧光团产生超过300种独特的签名。此外,从1296个时间分辨荧光签名,我们表明光学签名是重现的99.48 %的时间。同时检测多种生物实体的能力,高空间信息密度和合成RET网络的高可重复性可能在许多生物和临床应用中找到使用。

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