Ultrasensitive detection of disease biomarkers using an immuno-wall device with enzymatic amplification

Literature Information

Publication Date 2019-06-19
DOI 10.1039/C9AN00480G
Impact Factor 4.616
Authors

Keine Nishiyama, Seiya Nakamata, Koya Ishikawa, Masatoshi Maeki, Akihiko Ishida, Hirofumi Tani


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Abstract

We present an ultrasensitive immunoassay system for disease biomarkers utilizing the immuno-wall device and an enzymatic amplification reaction. The immuno-wall device consisted of 40 microchannels, each of which contained an antibody-modified wall-like structure along the longitudinal axis of the microchannel. The wall was fabricated with a water-soluble photopolymer containing streptavidin by photolithography, and biotinylated capture antibodies were immobilized on the sides through streptavidin–biotin interaction. For an assay, introducing the target biomarker and secondary and labeled antibodies produced a sandwich complex anchored on the sides of the wall. A conventional immuno-wall device uses a fluorescence-labeled antibody as a labeling antibody. To achieve an ultrasensitive detection of a trace biomarker, we used an enzyme label and amplified the signal with the enzymatic reaction with a fluorogenic substrate in the microchannel. The highest signal/background ratio was obtained by using alkaline phosphatase-labeled antibody and 9H-(1,3-dichloro-9,9-dimethylacridin-2-one-7-yl) phosphate. To evaluate the device performance, we detected human C-reactive protein (CRP) as a model biomarker. The detection limit (LOD) of CRP in phosphate-buffered saline was 2.5 pg mL−1 with a sample volume of 0.25 μL. This LOD was approximately 3 orders of magnitude lower than that obtained with fluorescent-dye (DyLight 650)-labeled antibody. In addition, the present device provided a wide detection range of 0.0025–10 ng mL−1 for CRP. We successfully developed an ultrasensitive immunoassay system with simple operation and only a small sample volume.

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Editorial

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DOI: 10.1039/JA988030299B

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David John Faulkner. 10th June 1942–23rd November 2002

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DOI: 10.1039/NP98603000I1

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