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Aptamer-based bio-barcode assay for the detection of cytochrome-c released from apoptotic cells |
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| Authors: | Irene P.M. Lau Jacky F.C. Loo H.P. Ho |
| Affiliation: | a Department of Biochemistry, The Chinese University of Hong Kong, Shatin, NT, Hong Kong b School of Biomedical Sciences, The Chinese University of Hong Kong, Shatin, NT, Hong Kong c Center for Advanced Research in Photonics, Department of Electronic Engineering, The Chinese University of Hong Kong, Shatin, NT, Hong Kong |
| Abstract: | The recently developed bio-barcode (BBC) assay using polymerase chain reaction (PCR) to generate signals has been shown to be an extraordinarily sensitive method to detect protein targets. The BBC assay involves a magnetic microparticle (with antibody to capture the target of interest) and gold nanoparticle (with recognition antibody and thiolated single-stranded barcode DNAs) to form a sandwich around the target. The concentration of target is determined by the amount of barcode DNA released from the nanoparticles. Here we describe a modification using aptamers to substitute the gold nanoparticles for the BBC assay. In this study, we isolated a 76-mer monoclonal aptamer against cytochrome-c (cyto-c) and this single-stranded DNA in defined 3D structure for cyto-c was used in the BBC assay for both recognition and readout reporting. After magnetic separation, the aptamer was amplified by PCR and this aptamer-based barcode (ABC) assay was sensitive enough to detect the cyto-c in culture medium released from the apoptotic cells after drug treatment at the picomolar level. When compared to the conventional cyto-c detection by Western blot analysis, our ABC assay is sensitive, and time for the detection and quantification with ready-made probes was only 3 h. |
| Keywords: | Aptamer Apoptosis Cytochrome-c Bio-barcode assay |
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