4.7 Article

Double-Antibody Sandwich Immunoassay and Plasmonic Coupling Synergistically Improved Long-Range SPR Biosensor with Low Detection Limit

Journal

NANOMATERIALS
Volume 11, Issue 8, Pages -

Publisher

MDPI
DOI: 10.3390/nano11082137

Keywords

nanophotonics; plasmonic detection; nanocomposite material; double-antibody sandwich immunoassay; plasmonic coupling between nano gold; low limit of detection

Funding

  1. National Natural Science Foundation of China [61922061, 61775161, 61735011]
  2. Tianjin Science Fund for Distinguished Young Scholars [19JCJQJC61400]
  3. National Instrument Program of China [2013YQ030915]

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The LR-SPR biosensor modified with double-antibody sandwich immunoassay and plasmonic coupling demonstrates high sensitivity and low LOD for human-IgG detection. The unique nanocomposite material in the sensor provides in situ self-compensation for disturbance, making it a valuable method for biochemical analysis and disease detection.
A long-range surface plasmonic resonance (LR-SPR) biosensor modified with double-antibody sandwich immunoassay and plasmonic coupling is demonstrated for human-immunoglobulin G detection with a low limit of detection (LOD). The double-antibody sandwich immunoassay dramatically changes the average refractive index of the medium layer on the sensor surface. The near-field electron coupling between the localized surface plasmon and the long-range surface plasmon leads to a significant perturbation of the evanescent field. The large penetration depth and the long propagation distance of the long-range surface plasmonic waves facilitate the LR-SPR sensor in the detection of biological macromolecules. The unique light absorption characteristic of the nanocomposite material in the sensor provides the in situ self-compensation for the disturbance. Therefore, besides the inherent advantages of optical fiber sensors, the developed biosensor can realize the detection of biomolecules with high sensitivity, low LOD and high accuracy and reliability. Experimental results demonstrate that the LOD of the biosensor is as low as 0.11 mu g/mL in the detection of the phosphate-buffered saline sample, and the spike-and-repetition rate is 105.56% in the detection of the real serum sample, which partly shows the practicability of the biosensor. This indicates that the LR-SPR biosensor provides better response compared with existing similar sensors and can be regarded as a valuable method for biochemical analysis and disease detection.

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