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纸张自发荧光的波长和寿命:一种简单的基底筛选工艺,可提高基于荧光的纸张分析方法的灵敏度。

Wavelengths and Lifetimes of Paper Autofluorescence: A Simple Substrate Screening Process to Enhance the Sensitivity of Fluorescence-Based Assays in Paper.

机构信息

Department of Bioengineering, University of Washington , Box 355061, Seattle, Washington 98195, United States.

出版信息

Anal Chem. 2017 Nov 21;89(22):12023-12029. doi: 10.1021/acs.analchem.7b02424. Epub 2017 Oct 31.

Abstract

Porous media made of nitrocellulose and glass fiber are common "paper" substrates for lateral flow assays, microfluidic paper analytical devices and other point-of-care diagnostic assays. Such assays commonly use optical labels such as gold nanoparticles, latex beads, or fluorescent nanoparticles to visualize the presence of analytes. Fluorescent labels are commonly used in bioassays to enhance sensitivity, but autoluminescence of the paper substrate worsens signal-to-noise ratios of fluorescence-based assays. To date, there exists no systematic investigation of autoluminescence wavelengths or lifetimes of porous membranes used in lateral flow assays. In response, we quantified the autoluminescence of commonly used porous materials across the visible spectrum via excitation-emission spectroscopy and time-resolved fluorescence spectroscopy, and demonstrate that autoluminescence is solely due to autofluorescence with lifetimes of about 5 ns in the visible spectrum. Counterintuitively, we found that spectroscopy alone does not provide sufficient information to select candidate paper substrates for fluorophore-labeled assays. Therefore, we developed a simple quantitative framework to select a low-fluorescence substrate that minimizes both the overlap of paper and fluorophore emission spectra and the fluorescence intensity on an imaging system of interest (such as a gel imager). Use of this framework was shown to lower the limit of detection of an influenza A nucleoprotein immunoassay by over 50%. The tools developed in this manuscript enable assay developers to screen appropriate, low-fluorescence porous substrates and enhance the sensitivity of membrane-based fluorescence assays.

摘要

由硝化纤维素和玻璃纤维制成的多孔介质是侧向流动分析、微流控纸分析装置和其他即时诊断分析的常见“纸”基底。此类分析通常使用光学标记物,如金纳米粒子、乳胶珠或荧光纳米粒子,来可视化分析物的存在。荧光标记物通常用于生物测定以提高灵敏度,但纸基底的自发光会降低基于荧光的测定的信噪比。迄今为止,尚无针对侧向流动分析中使用的多孔膜的自发光波长或寿命的系统研究。有鉴于此,我们通过激发-发射光谱法和时间分辨荧光光谱法对常见的多孔材料在整个可见光谱范围内的自发光进行了量化,并证明自发光仅归因于在可见光谱中具有约 5 ns 寿命的自发荧光。具有讽刺意味的是,我们发现仅凭光谱学无法提供足够的信息来选择适合荧光标记分析的候选纸基底。因此,我们开发了一种简单的定量框架来选择低荧光基底,该框架可最大限度地减少纸和荧光团发射光谱的重叠以及感兴趣的成像系统(如凝胶成像仪)上的荧光强度。该框架的使用表明,流感 A 核蛋白免疫测定的检测限降低了 50%以上。本文档中开发的工具使分析开发人员能够筛选合适的低荧光多孔基底,并提高基于膜的荧光分析的灵敏度。

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