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首页> 外文期刊>Journal of chromatography, A: Including electrophoresis and other separation methods >Feasibility of asymmetrical flow field-flow fractionation as a method for detecting protective antigen by direct recognition of size-increased target-captured nanoprobes
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Feasibility of asymmetrical flow field-flow fractionation as a method for detecting protective antigen by direct recognition of size-increased target-captured nanoprobes

机译:通过直接识别尺寸增大的目标捕获纳米探针来检测保护性抗原的方法,不对称流场-流分馏的可行性

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摘要

Asymmetrical flow field-flow fractionation (AF4) was evaluated as a potential analytical method for detection of a protective antigen (PA), an Anthrax biomarker. The scheme was based on the recognition of altered AF4 retention through the generation of the size-increased Au nanoparticle probes as a result of PA binding, in which a PA-selective peptide was conjugated on the probe surface. In the visible absorption-based AF4 fractograms, the band position shifted to a longer retention time as the PA concentration increased due to the presence of probe bound with PAs. The shift was insignificant when the concentration was relatively low at 84.3 pM. To improve sensitivity, two separate probes conjugated with two different peptides able to bind on different PA epitopes were used together. The band shift then became distinguishable even at 84.3 pM of PA sample. The formation of larger PA-probe inter-connected species using the dual-probe system was responsible for the enhanced band shift. In parallel, the feasibility of surface-enhanced Raman scattering (SERS) as a potential AF4 detection method was also evaluated. In the off-line SERS fractogram constructed using fractions collected during AF4 separation, a band shift was also observed for the 84.3 pM PA sample, and the band intensity was higher when using the dualprobe system. The combination of AF4 and SERS is promising for the detection of PA and will become a potential tool if the reproducibility of SERS measurement is improved. (C) 2015 Elsevier B.V. All rights reserved.
机译:评价不对称流场流分离(AF4)作为检测保护性抗原(PA)(一种炭疽生物标志物)的潜在分析方法。该方案基于通过PA结合而生成的尺寸增大的Au纳米颗粒探针,从而识别出AF4保留的改变,其中PA结合是在探针表面缀合了PA选择肽。在基于可见光的AF4形貌图中,随着PA浓度的增加,由于存在与PA结合的探针,谱带位置移动到更长的保留时间。当浓度相对较低时仅为84.3 pM,变化不明显。为了提高灵敏度,将结合了两个能够与不同PA表位结合的不同肽结合的单独探针一起使用。然后即使在PA样品为84.3 pM时,带移也变得可分辨。使用双探针系统形成更大的PA探针互连物种是增强的带移的原因。同时,还评估了表面增强拉曼散射(SERS)作为潜在的AF4检测方法的可行性。在使用AF4分离过程中收集的馏分构建的离线SERS分数图中,也观察到了84.3 pM PA样品的带移,并且使用双探针系统时,带强度更高。 AF4和SERS的组合有望用于PA的检测,如果提高SERS测量的可重复性,它将成为潜在的工具。 (C)2015 Elsevier B.V.保留所有权利。

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