Towards the Development of a 3-D Biochip for the Detection of Hepatitis C Virus

The early diagnostics of hepatitis C virus (HCV) infections is currently one of the most highly demanded medical tasks. This study is devoted to the development of biochips (microarrays) that can be applied for the detection of HCV. The analytical platforms of suggested devices were based on macropo...

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Published inSensors (Basel, Switzerland) Vol. 20; no. 9; p. 2719
Main Authors Antipchik, Mariia, Polyakov, Dmitry, Sinitsyna, Ekaterina, Dzhuzha, Apollinariia, Shavlovsky, Mikhail, Korzhikova-Vlakh, Evgenia, Tennikova, Tatiana
Format Journal Article
LanguageEnglish
Published Switzerland MDPI AG 10.05.2020
MDPI
Subjects
Antibodies
Antigens
Bioassays
Biochips
Blood plasma
Buffer solutions
Chromatography
Enzymes
Hepacivirus
Hepatitis
Hepatitis C
Hepatitis C - diagnosis
Humans
Immunoassay
Ligands
macroporous monolithic polymer layers
microarray
Microarray Analysis
Monolithic materials
Polymerization
Polymers
Pore size
Proteins
Reproducibility of Results
Systems analysis
virus-mimetic particles
Viruses
United States > US
Germany
Russia
biochips
microarray
macroporous monolithic polymer layers
hepatitis C
virus-mimetic particles
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Summary:The early diagnostics of hepatitis C virus (HCV) infections is currently one of the most highly demanded medical tasks. This study is devoted to the development of biochips (microarrays) that can be applied for the detection of HCV. The analytical platforms of suggested devices were based on macroporous poly(glycidyl methacrylate- -di(ethylene glycol) dimethacrylate) monolithic material. The biochips were obtained by the covalent immobilization of specific probes spotted onto the surface of macroporous monolithic platforms. Using the developed biochips, different variants of bioassay were investigated. This study was carried out using hepatitis C virus-mimetic particles (VMPs) representing polymer nanoparticles with a size close to HCV and bearing surface virus antigen (E2 protein). At the first step, the main parameters of bioassay were optimized. Additionally, the dissociation constants were calculated for the pairs "ligand-receptor" and "antigen-antibody" formed at the surface of biochips. As a result of this study, the analysis of VMPs in model buffer solution and human blood plasma was carried out in a format of direct and "sandwich" approaches. It was found that bioassay efficacy appeared to be similar for both the model medium and real biological fluid. Finally, limit of detection (LOD), limit of quantification (LOQ), spot-to-spot and biochip-to-biochip reproducibility for the developed systems were evaluated.
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ISSN:1424-8220
1424-8220
DOI:10.3390/s20092719