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Label-less fluorescence-based method to detect hybridization with applications to DNA micro-array

机译:基于无标记荧光的检测杂交的方法及其在DNA微阵列中的应用

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By coupling scattered light from DNA to excite fluorescence in a polymer, we describe a quantitative, label-free assay for DNA hybridization detection. Since light scattering is intrinsically proportional to number of molecules, the change in (scattering coupled) fluorescence is highly linear with respect to percent binding of single stranded DNA (ssDNA) target with the immobilized ssDNA probes. The coupling is achieved by immobilizing ssDNA on a fluorescent polymer film at optimum thickness in nanoscale. The fluorescence from the underlining polymer increases due to proportionate increase in scattering from double stranded DNA (dsDNA) (i.e., probe-target binding) compared to ssDNA (i.e., probe). Because the scattering is proportional to fourth power of refractive index, the detection of binding is an order of magnitude more sensitive compared to other label-free optical methods, such as, reflectivity, interference, ellipsometry and surface-plasmon resonance. Remarkably, polystyrene film of optimum thickness 30 nm is the best fluorescent agent since its excitation wavelength matches (within 5 nm) with wavelength for the maximum refractive index difference between ssDNA and dsDNA. A quantitative model (with no fitting parameters) explains the observations. Potential dynamic range is 1 in 10(4) at signal-to-noise ratio of 3: 1. (c) 2007 Elsevier B.V. All rights reserved.
机译:通过耦合来自DNA的散射光以激发聚合物中的荧光,我们描述了DNA杂交检测的定量,无标记测定。由于光散射本质上与分子数量成正比,因此(散射耦合)荧光的变化相对于单链DNA(ssDNA)靶标与固定的ssDNA探针的结合百分比呈高度线性关系。通过将ssDNA固定在荧光聚合物薄膜上,达到纳米级的最佳厚度,即可实现偶联。与ssDNA(即探针)相比,由于来自双链DNA(dsDNA)的散射成比例增加(即探针与靶标结合),来自下划线聚合物的荧光增加。由于散射与折射率的四次方成正比,因此与其他无标记的光学方法(例如,反射率,干涉,椭圆光度法和表面等离子体共振)相比,结合的检测更加灵敏一个数量级。值得注意的是,最佳厚度为30 nm的聚苯乙烯薄膜是最好的荧光剂,因为它的激发波长与ssDNA和dsDNA之间最大折射率差的波长匹配(在5 nm内)。定量模型(没有拟合参数)解释了观察结果。潜在的动态范围是10(4)中的1,信噪比为3:1。(c)2007 Elsevier B.V.保留所有权利。

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