Abstract

A novel strategy is presented for sensitive detection of alfa-fetoprotein (AFP), using a horseradish peroxidase (HRP)-functionalized Envision antibody complex (EVC) as the label. The Envision-AFP signal antibody copolymer (EVC-AFP Ab2) was composed of a dextran amine skeleton anchoring more than 100 molecules of HRP and 15 molecules of secondary antibody, and acted as a signal tag in the immunosensor. The sensor was constructed using the following steps: First, gold electrode (GE) was modified with nano-gold (AuNPs) by electro-deposition in HAuCl4 solution. The high affinity of the AuNPs surface facilitates direct formation of a self-assembled thiolated protein G layer. Next, the coated GE was incubated in a solution of AFP capture antibody (AFP Ab1); these antibodies attach to the thiolated protein G layer through their non-antigenic regions, leaving the antigen binding sites for binding of target analyte. Following a sandwich immunoreaction, an EVC-AFP Ab2-AFP-AFP Ab1 immunocomplex was formed on the electrode surface, allowing large amounts of HRP on the complex to produce an amplified electrocatalytic current of hydroquinone (HQ) in the presence of hydrogen peroxide (H2O2). Highly amplified detection was achieved, with a detection limit of 2 pg/mL and a linear range of 0.005–0.2 ng/mL for AFP in 10 μL undiluted serum; this is near or below the normal levels of most cancer biomarker proteins in human serum. Measurements of AFP in the serum of cancer patients correlated strongly with standard enzyme-linked immunosorbent assays. These easily fabricated EVC-modified immunosensors show excellent promise for future fabrication of bioelectronic arrays. By varying the target biomolecules, this technique may be easily extended for use with other immunoassays, and thus represents a versatile design route.

Highlights

  • Alfa-fetoprotein (AFP), a glycoprotein with a molecular weight of about 70,000 Da, is used as a serum-based marker for several types of malignant neoplasm, including hepatic and yolk sac tumors [1,2,3].Sensitive detection of AFP is crucial for many areas of modern biochemical and biomedical research, providing opportunities for understanding the fundamental biological processes involved in disease progression, and for monitoring the patient response to therapy

  • After reacting AFP Ab1 with thiolated protein G, the corresponding scanning electron microscopy (SEM) image showed a flat protein membrane spread over the electrode

  • These results indicate that the Envision antibody complex (EVC) had been successfully prepared using AFP Ab2 and horseradish peroxidase (HRP)

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Summary

Introduction

Alfa-fetoprotein (AFP), a glycoprotein with a molecular weight of about 70,000 Da, is used as a serum-based marker for several types of malignant neoplasm, including hepatic and yolk sac tumors [1,2,3]. Our present work on an electrochemical immunosensor for AFP detection, based on nano-gold (AuNPs) and EVC-AFP Ab2 bioconjugates to achieve ultrasensitive signal amplification, was developed to verify the amplification process of enzyme-functionalized nanoparticles. Enhanced detection sensitivity was obtained using multi-labeled bioconjugates, with multiple HRP molecules linked to the EVC-AFP Ab2 signal tag for signal development Using this approach, we obtained enriched enzyme loading in each sandwich immunological reaction, which subsequently enhanced the electrocatalytic current measured for detection of AFP protein. We obtained enriched enzyme loading in each sandwich immunological reaction, which subsequently enhanced the electrocatalytic current measured for detection of AFP protein This simple, cost-effective and sensitive immunosensor would have the ability to detect most cancer biomarker proteins in human serum at levels near or below the normal range, and could be used in clinical analysis for a wide range of potential applications

Morphological Characterization of the Envision Nanocomposite
Electrochemical Characterization of the Immunosensor
Optimization of Experimental Conditions
Calibration Curve of the Immunosensor
Regeneration of the Immunosensor
Apparatus and Regents
Preparation of Thiolated Protein G Modified Au Electrode
Fabrication of the Immunosensor
Electrochemical Measurements of AFP
Conclusions
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