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Improving the Instrumental Resolution of Sensors Based on Localized Surface Plasmon Resonance

机译:基于局部表面等离振子共振提高传感器的仪器分辨率

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The colorimetric variations induced upon changes in interfacial refractive index of nanoscale noble metal structures exhibiting localized surface plasmon resonance (LSPR) provides a convenient means of label-free, affinity-based detection of biomolecular recognition reactions. However, despite being similar in nature to conventional SPR, LSPR has so far suffered from significantly lower data quality in terms of its signal-to-noise ratio (S/N) in typical biomolecular recognition analysis. In this work, generic data analysis algorithms and a simple experimental setup that provide a S/N upon protein binding that is comparable to that of state-of-the art SPR systems are presented. Specifically, it is demonstrated how temporal variations (rate approx0.5 Hz) in parameters proportional to the resonance peak position can be recorded simultaneously, yielding a peak position precision of <5 X 10~(-4) nm and an extinction noise level of <5 X 10~(-6) absorbance units (Abs). This, in turn, is shown to provide a S/N of approx2000 (equivalent to a detection limit of <0.1 ng/cm~(2)) for typical protein binding reactions. Furthermore, the importance of utilizing changes in both peak position and magnitude is highlighted by comparing different LSPR active noble metal architectures that respond differently to bulk and interfacial refractive index changes.
机译:在表现出局部表面等离子体共振(LSPR)的纳米级贵金属结构的界面折射率变化时引起的比色变化为生物分子识别反应的无标记,基于亲和力的检测提供了方便的手段。然而,尽管LSPR本质上与常规SPR相似,但到目前为止,在典型的生物分子识别分析中,LSPR的信噪比(S / N)明显降低了数据质量。在这项工作中,提出了通用的数据分析算法和一个简单的实验设置,可以在蛋白质结合后提供S / N,可与最新的SPR系统相媲美。具体而言,证明了如何同时记录与共振峰位置成正比的参数的时间变化(速率约0.5 Hz),从而产生<5 X 10〜(-4)nm的峰位置精度和消声水平为。 <5 X 10〜(-6)吸光度单位(Abs)。反过来,对于典型的蛋白质结合反应,这显示出提供了大约2000的S / N(相当于<0.1 ng / cm〜(2)的检测极限)。此外,通过比较不同的LSPR活性贵金属体系结构(对体积和界面折射率变化有不同的响应),强调了利用峰位置和幅度变化的重要性。

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