Aptamer-functionalized nanoparticles for surface immobilization-free electrochemical detection of cortisol in a microfluidic device

被引:147
作者
Sanghavi, Bankim J. [1 ]
Moore, John A. [1 ]
Chavez, Jorge L. [2 ]
Hagen, Joshua A. [2 ]
Kelley-Loughnane, Nancy [2 ]
Chou, Chia-Fu [3 ]
Swami, Nathan S. [1 ]
机构
[1] Univ Virginia, Dept Elect & Comp Engn, Charlottesville, VA 22904 USA
[2] Human Effectiveness Directorate, Air Force Res Lab, 711th Human Performance Wing, Dayton, OH 45433 USA
[3] Acad Sinica, Inst Phys, Taipei 11529, Taiwan
关键词
Aptamer; Cortisol; Microfluidics; Nanoslit; Voltammetry; GRAPHENE-MODIFIED ELECTRODES; CAPILLARY-ELECTROPHORESIS; NANOFLUIDIC CHANNELS; PHYSIOLOGICAL MEDIA; PLASMA-CORTISOL; PERFORMANCE; RADIOIMMUNOASSAY; IMMUNOASSAY; SYSTEM; PRECONCENTRATION;
D O I
10.1016/j.bios.2015.11.044
中图分类号
Q6 [生物物理学];
学科分类号
071011 ;
摘要
Monitoring the periodic diurnal variations in cortisol from small volume samples of serum or saliva is of great interest, due to the regulatory role of cortisol within various physiological functions and stress symptoms. Current detection assays are immunologically based and require cumbersome antibody immobilization chemistries, thereby limiting the assay versatility, kinetics, and reproducibility. We present a quantitative aptamer-based detection methodology for cortisol that does not require target labeling, capture probe immobilization on the detection surface or wash steps prior to readout. Using a recognition system of aptamer functionalized gold nanoparticles pre-bound with electro-active triamcinolone, the cortisol level is detected based on its competitive binding to the aptamer by following signal from the displaced triamcinolone using square wave voltammetry at patterned graphene-modified electrodes in a microfluidic or nanoslit device. Due to the 3D analyte diffusion profile at the aptamer interface and the ability to enhance the surface area for cortisol capture, this assay shows signal linearity over a five-log analyte concentration range (10 mu g/mL to 30 pg/mL) and exhibits rapid binding kinetics with cortisol versus other glucocorticoids, as apparent from the absence of interferences from estradiol, testosterone and progesterone. The assay is carried out within the biologically relevant range for glucocorticoids in serum and saliva matrices, and benchmarked versus ELISA and radioimmunoassays. Based on absence of cumbersome surface immobilization and wash steps for carrying out this assay, its quantitative signal characteristics and its ability to resist interferences from other glucocorticoids, we envision its application towards routine monitoring of cortisol within bio-fluids. (C) 2015 Elsevier B.V. All rights reserved.
引用
收藏
页码:244 / 252
页数:9
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