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用生物素和辣根过氧化物酶标记的脂质体:一种通过在电极上沉淀不溶性产物来增强抗原-抗体或寡核苷酸- DNA传感过程放大作用的探针。

Liposomes labeled with biotin and horseradish peroxidase: a probe for the enhanced amplification of antigen--antibody or oligonucleotide--DNA sensing processes by the precipitation of an insoluble product on electrodes.

作者信息

Alfonta L, Singh A K, Willner I

机构信息

The Institute of Chemistry, The Hebrew University of Jerusalem, Israel.

出版信息

Anal Chem. 2001 Jan 1;73(1):91-102. doi: 10.1021/ac000819v.

Abstract

Liposomes labeled with biotin and the enzyme horseradish peroxidase (HRP) are used as a probe to amplify the sensing of antigen-antibody interactions or oligonucleotide-DNA binding. The HRP-biocatalyzed oxidation of 4-chloro-1-naphthol (1) in the presence of H2O2, and the precipitation of the insoluble product 2 on electrode supports, are used as an amplification route for the sensing processes. The anti-dinitrophenyl antibody (DNP-Ab) is sensed by a dinitrophenyl-L-cysteine antigen monolayer associated with an Au electrode. A biotinylated anti-IgG-antibody (Fc-specific) is linked to the antigen-DNP-Ab complex, and the biotin-labeled HRP-liposomes associate with the assembly through an avidin bridge. The biocatalyzed precipitation of 2 on the electrode increases the electron-transfer resistances at the electrode-solution interface or the electrode resistance itself. The binding events of the different proteins on the electrode and the biocatalyzed precipitation of 2 on the conductive support are followed by Faradaic impedance spectroscopy or constant-current chronopotentiometry. DNP-Ab concentrations as low as 1 x 10(-11) g x mL(-1) can be detected by this method. The labeled liposomes were also used for the amplified detection of DNA 3. The oligonucleotide 4, complementary to a part of the target DNA 3 that is a model nucleic acid sequence for the Tay-Sachs genetic disorder, is assembled on an Au electrode. Hybridization of the analyte 3 followed by the association of the biotin-tagged oligonucleotide 5 yields a three-component double-stranded assembly. Sensing of the analyte 3 is amplified by the association of avidin, the labeled liposomes, and the subsequent biocatalyzed precipitation of 2 on the electrodes. The DNA 3 is detected with a sensitivity that corresponds to 6.5 x 10(-13) M. Faradaic impedance spectroscopy and chronopotentiometry were employed to follow the stepwise assembly of the systems and the electronic transduction of the detection of the analyte DNA 3.

摘要

用生物素和辣根过氧化物酶(HRP)标记的脂质体作为探针,用于放大对抗抗原 - 抗体相互作用或寡核苷酸 - DNA结合的传感。在H2O2存在下,HRP催化4 - 氯 - 1 - 萘酚(1)的氧化,以及不溶性产物2在电极载体上的沉淀,用作传感过程的放大途径。通过与金电极相关联的二硝基苯基 - L - 半胱氨酸抗原单层来传感抗二硝基苯基抗体(DNP - Ab)。生物素化的抗IgG抗体(Fc特异性)与抗原 - DNP - Ab复合物相连,并且生物素标记的HRP - 脂质体通过抗生物素蛋白桥与该组装体结合。2在电极上的生物催化沉淀增加了电极 - 溶液界面处的电子转移电阻或电极本身的电阻。通过法拉第阻抗谱或恒流计时电位法跟踪不同蛋白质在电极上的结合事件以及2在导电载体上的生物催化沉淀。该方法可检测低至1×10(-11)g×mL(-1)的DNP - Ab浓度。标记的脂质体还用于DNA 3的放大检测。与作为泰 - 萨克斯遗传病模型核酸序列的靶DNA 3的一部分互补的寡核苷酸4组装在金电极上。分析物3杂交后,生物素标记的寡核苷酸5缔合,产生三组分双链组装体。通过抗生物素蛋白、标记的脂质体的缔合以及随后2在电极上的生物催化沉淀来放大对分析物3的传感。检测到的DNA 3的灵敏度对应于6.5×10(-13)M。采用法拉第阻抗谱和计时电位法跟踪系统的逐步组装以及分析物DNA 3检测的电子转导。

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