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Iodine-Mediated Etching of Gold Nanorods for Plasmonic ELISA Based on Colorimetric Detection of Alkaline Phosphatase

机译:基于碱性磷酸酶比色检测的碘介导的金纳米棒的等离子蚀刻蚀刻。

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摘要

Here, we propose a plasmonic enzyme-linked immunosorbent assay (ELISA) based on highly sensitive colorimetric detection of alkaline phosphatase (ALP), which is achieved by iodine-mediated etching of gold nanorods (AuNRs). Once the sandwich-type immunocomplex is formed, the ALP bound on the polystyrene microwells will hydrolyze ascorbic acid 2-phosphate into ascorbic acid. Subsequently, iodate is reduced to iodine, a moderate oxidant, which etches AuNRs from rod to sphere in shape. The shape change of AuNRs leads to a blue-shift of longitudinal localized surface plasmon resonance. As a result, the solution of AuNRs changes from blue to red. Benefiting from the highly sensitive detection of ALP, the proposed plasmonic ELISA has achieved an ultralow detection limit (100 pg/mL) for human immunoglobulin G (IgG). Importantly, the visual detection limit (3.0 ng/mL) allows the rapid differential diagnosis with the naked eye. The further detection of human IgG in fetal bovine serum indicates its applicability to the determination of low abundance protein in complex biological samples.
机译:在这里,我们提出了一种基于碱性磷酸酶(ALP)的高灵敏度比色检测的等离激元酶联免疫吸附测定(ELISA),该检测是通过碘介导的金纳米棒(AuNRs)蚀刻实现的。一旦形成夹心型免疫复合物,结合在聚苯乙烯微孔上的ALP会将抗坏血酸2-磷酸水解为抗坏血酸。随后,碘酸盐还原为碘,一种中等氧化剂,将AuNRs从棒状蚀刻到球形。 AuNRs的形状变化导致纵向局部表面等离子体激元共振的蓝移。结果,AuNR的解从蓝色变为红色。得益于对ALP的高度灵敏检测,拟议的等离子ELISA已达到人免疫球蛋白G(IgG)的超低检测限(100 pg / mL)。重要的是,视觉检测极限(3.0 ng / mL)可以用肉眼快速鉴别诊断。胎儿牛血清中人IgG的进一步检测表明其可用于测定复杂生物样品中的低丰度蛋白。

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