4.7 Article

Aptamer/antibody sandwich method for digital detection of SARS-CoV2 nucleocapsid protein

TALANTA (2022)

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Journal

TALANTA
Volume 236, Issue -, Pages -

Publisher

ELSEVIER
DOI: 10.1016/j.talanta.2021.122847

Keywords

Digital detection; Microfluidic chip; COVID-19; SARS-CoV2; Nucleocapsid protein; Aptamer/antibody sandwich

Categories

Chemistry, Analytical

Funding

  1. Special anti-COVID-19 Project Fund of Guangdong Provincial Education Department [2020KZDZX1214]
  2. Natural Science Foundation of Top Talent of SZTU [2020102]
  3. Shenzhen Natural Science Foundation [JCYJ20190813141001745]
  4. Startup Research Fund of Shenz-hen Technology University
  5. Shenzhen Pengcheng Scholar Program
  6. Special Fund for Science and Technology Innovation of Pingshan District, Shenzhen [PSKG202006]

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A microfluidic chip with femtoliter-sized wells was developed for sensitive digital detection of the N protein in SARS-CoV2. This method showed a detection limit of 33.28 pg/mL, which was 300 times lower than traditional ELISA, making it an accurate tool for early diagnosis of SARS-CoV2.
Nucleocapsid protein (N protein) is the most abundant protein in SARS-CoV2 and is highly conserved, and there are no homologous proteins in the human body, making it an ideal biomarker for the early diagnosis of SARS-CoV2. However, early detection of clinical specimens for SARS-CoV2 remains a challenge due to false-negative results with viral RNA and host antibodies based testing. In this manuscript, a microfluidic chip with femtoliter-sized wells was fabricated for the sensitive digital detection of N protein. Briefly, beta-galactosidase (beta-Gal)-linked antibody/N protein/aptamer immunocomplexes were formed on magnetic beads (MBs). Afterwards, the MBs and beta-Gal substrate fluorescein-di-beta-D-galactopyranoside (FDG) were injected into the chip together. Each well of the chip would only hold one MB as confined by the diameter of the wells. The MBs in the wells were sealed by fluorocarbon oil, which confines the fluorescent (FL) product generated from the reaction between beta-Gal and FDG in the individual femtoliter-sized well and creates a locally high concentration of the FL product. The FL images of the wells were acquired using a conventional inverted FL microscope. The number of FL wells with MBs (FL wells number) and the number of wells with MBs (MBs wells number) were counted, respectively. The percentage of FL wells was calculated by dividing (FL wells number) by (MBs wells number). The higher the percentage of FL wells, the higher the N protein concentration. The detection limit of this digital method for N protein was 33.28 pg/mL, which was 300 times lower than traditional double-antibody sandwich based enzyme-linked immunosorbent assay (ELISA).

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