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Affinity Peptide-Tethered Suspension Hydrogel Sensor for Selective and Sensitive Detection of Influenza Virus

Authors
Kim, Ji HongJeong, Hye-SeonHwang, JaehyeonKweon, Dae-HyukChoi, Chang-HyungPark, Jong Pil
Issue Date
Oct-2023
Publisher
AMER CHEMICAL SOC
Keywords
phage display; peptide; hydrogel microsphere; fluorescence sensor
Citation
ACS APPLIED MATERIALS & INTERFACES, v.15, no.44, pp 52051 - 52064
Pages
14
Journal Title
ACS APPLIED MATERIALS & INTERFACES
Volume
15
Number
44
Start Page
52051
End Page
52064
URI
https://scholarworks.bwise.kr/cau/handle/2019.sw.cau/70222
DOI
10.1021/acsami.3c14470
ISSN
1944-8244
1944-8252
Abstract
Influenza viruses are known to cause pandemic flu outbreaks through both inter-human and animal-to-human transmissions. Therefore, the rapid and accurate detection of such pathogenic viruses is crucial for effective pandemic control. Here, we introduce a novel sensor based on affinity peptide-immobilized hydrogel microspheres for the selective detection of influenza A virus (IAV) H3N2. To enhance the binding affinity performance, we identified novel affinity peptides using phage display and further optimized their design. The functional hydrogel microspheres were constructed using the drop microfluidic technique, employing a structure composed of natural (chitosan) and synthetic (poly(ethylene glycol) diacrylate and PEG 6 kDa) polymers with the activation of azadibenzocyclooctyne for the subsequent click chemistry reaction. The binding peptide-immobilized hydrogel microsphere (BP-Hyd) was characterized by field emission scanning electron microscopy, X-ray photoelectron spectroscopy, and Fourier transform infrared spectroscopy and exhibited selective detection capability for the IAV H3N2. To capture the detected IAV H3N2, a Cy3-labeled IAV hemagglutinin antibody was utilized. By incorporating the affinity peptide with hydrogel microspheres, we achieved quantitative and selective detection of IAV H3N2 with a detection limit of 1.887 PFU mL(-1). Furthermore, the developed suspension sensor exhibited excellent reproducibility and showed reusability potential. Our results revealed that the BP-Hyd-based fluorescence sensor platform could be feasibly employed to detect other pathogens because the virus-binding peptides can be easily replaced with other peptides through phage display, enabling selective and sensitive binding to different targets.
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