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通过凝血酶诱导纳米粒子纳入纤维蛋白来抑制纤维蛋白原稳定的金纳米粒子的催化活性:用于凝血酶检测的 10 倍以上选择性的应用。

Inhibition of catalytic activity of fibrinogen-stabilized gold nanoparticles via thrombin-induced inclusion of nanoparticle into fibrin: Application for thrombin sensing with more than 10-fold selectivity.

机构信息

Department of Chemistry, National Sun Yat-sen University, Taiwan.

Department of Applied Physics and Chemistry, University of Taipei, Taiwan.

出版信息

Spectrochim Acta A Mol Biomol Spectrosc. 2019 Mar 5;210:59-65. doi: 10.1016/j.saa.2018.11.013. Epub 2018 Nov 9.

DOI:10.1016/j.saa.2018.11.013
PMID:30445261
Abstract

Citrate-capped gold nanoparticles (AuNPs) modified with thrombin-binding aptamer are often implemented for colorimetric, fluorescent, and electrochemical detection of thrombin in an aqueous solution. However, researchers have rarely explored the application of fibrinogen-modified AuNPs (F-AuNPs) for thrombin sensing. We present a simple, inexpensive, sensitive, and selective probe for colorimetric assay of thrombin through combining thrombin-induced inclusion of F-AuNPs into Fibrin and F-AuNPs-catalyzed reduction of 4-nitrophenol with an excess amount of NaBH. Considering that fibrinogen stabilized citrate-capped AuNPs against a high-ionic-strength buffer, F-AuNPs efficiently catalyzed the NaBH-mediated decrease of yellow 4-nitrophenol to colorless 4-aminophenol. The presence of thrombin converted fibrinogen into fibrin on the nanoparticle surface, leading to the inclusion of nanoparticles into fibrin. The formation of fibrin inhibited that the AuNPs catalyzed the NaBH-mediated reduction of 4-nitrophenol. Consequently, the color of the solution gradually varied from colorless to yellow with increasing thrombin concentration. The proposed system was shown to be accurate in the quantification of small differences in the concentration of human thrombin over the range of 4-60 pM. The lowest detectable concentration of human thrombin by the naked eye was as low as 16 pM. We demonstrated the practical application of the proposed system in quantifying 1-15 nM human thrombin in human plasma.

摘要

金纳米粒子(AuNPs)被柠檬酸钠稳定后,通过与凝血酶结合适配体进行修饰,常被应用于水溶液中凝血酶的比色、荧光和电化学检测。然而,研究者很少探索纤维蛋白原修饰的 AuNPs(F-AuNPs)在凝血酶传感方面的应用。我们提出了一种简单、廉价、灵敏且选择性的比色法探针,用于凝血酶的检测。该探针通过将 F-AuNPs 结合到纤维蛋白中,以及 F-AuNPs 催化过量的 NaBH 将 4-硝基苯酚还原,实现了凝血酶的比色检测。考虑到纤维蛋白原可以稳定柠檬酸钠稳定的 AuNPs 免受高离子强度缓冲液的影响,F-AuNPs 可以有效地催化 NaBH 介导的黄色 4-硝基苯酚还原为无色 4-氨基酚。凝血酶的存在将纤维蛋白原转化为纳米颗粒表面的纤维蛋白,导致纳米颗粒被包含在纤维蛋白中。纤维蛋白的形成抑制了 AuNPs 催化 4-硝基苯酚被 NaBH 还原。因此,随着凝血酶浓度的增加,溶液的颜色逐渐从无色变为黄色。该体系在 4-60 pM 范围内对人凝血酶浓度的微小差异进行定量分析时,表现出了很高的准确性。通过肉眼检测人凝血酶的最低检测浓度低至 16 pM。我们证明了该体系在人血浆中定量检测 1-15 nM 人凝血酶的实际应用。

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