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One-Step Immunoassay for the Detection of Influenza Virus Based on Screened Nucleoprotein (NP)-like Mimotopes from Fv-Antibody LibraryOne‑Step Immunoassay for the Detection of Influenza Virus Based on Screened Nucleoprotein (NP)‑like Mimotopes from Fv‑Antibody Library

Other Titles
One‑Step Immunoassay for the Detection of Influenza Virus Based on Screened Nucleoprotein (NP)‑like Mimotopes from Fv‑Antibody Library
Authors
Kim, Tae-HunJung, JaeyongSung, Jeong SooKwon, SoonilBae, Hyung EunShim, Won-BoKang, Min-JungJose, JoachimPyun, Jae-Chul
Issue Date
Mar-2025
Publisher
한국바이오칩학회
Keywords
Fv-antibody library; Screening; Nucleoprotein (NP); Mimotope; One-step immunoassay; Influenza virus
Citation
BioChip Journal, v.19, no.1, pp 117 - 132
Pages
16
Indexed
SCIE
SCOPUS
KCI
Journal Title
BioChip Journal
Volume
19
Number
1
Start Page
117
End Page
132
URI
https://scholarworks.gnu.ac.kr/handle/sw.gnu/75647
DOI
10.1007/s13206-024-00185-9
ISSN
1976-0280
2092-7843
Abstract
The nucleoprotein (NP)-like mimotopes of influenza-A (Inf-A) virus were screened from autodisplayed Fv-antibody library and these NP-like mimotopes were applied to one-step immunoassay of influenza virus. The NP-like mimotopes were screened from an Fv-antibody library. The Fv-antibody represented the V-H region of heavy chain IgG, and the Fv-antibody library was prepared by randomizing CDR3 region. Therefore, prepared Fv-antibody library was expressed on the outer membrane of Escherichia coli using autodisplay technology. The target Fv-antibodies with the binding affinity to anti-NP monoclonal antibody (mAb) for Inf-A were screened as the NP-like mimotopes, and four clones were screened to have with the binding affinity to anti-NP mAb. The screened Fv-antibodies (NP-like mimotopes) were expressed as fusion proteins with a super folder green fluorescent protein (sfGFP), and the binding affinity (K-D) of NP-like mimotopes was estimated using SPR biosensors. The one-step immunoassay was configured for detecting Inf-A NP by binding NP-like mimotopes to immobilized anti-NP mAbs. The NP-like mimotopes (labeled with sfGFP) were quantitatively dissociated when the Inf-A NP (target analyte) were bound to immobilized anti-NP mAbs. The one-step immunoassay based on NP-like mimotopes was estimated to have a far higher sensitivity than the conventional lateral-flow immunoassay. Additionally, the one-step immunoassay for Inf-A was determined to be used for the detection of influenza-B (Inf-B) because of a high similarity (> 70%) in the amino acid sequence of NPs of Inf-A and Inf-B. Using the real samples of Inf-A and Inf-B (both were heat deactivated), the one-step immunoassay was demonstrated to be feasible for the medical diagnosis of Inf-A as well as Inf-B.
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농업생명과학대학 (식품공학부)
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