Production of a polyclonal antibody against acrylamide for immunochromatographic detection of acrylamide using strip tests
Objective: To produce, purify, and characterize a polyclonal antibody against acrylamide (anti-AA) for an application to immunochromatographic strip tests for AA. Material and Methods: Polyclonal anti-AA was prepared by injecting N-acryloxysuccinimide-conjugated bovine serum albumin hapten-antigen...
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Network for the Veterinarians of Bangladesh
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doaj-312f5adab7964788a57f71f0ce68e68a2020-11-24T21:36:02ZengNetwork for the Veterinarians of BangladeshJournal of Advanced Veterinary and Animal Research2311-77102019-09-016336637510.5455/javar.2019.f35639101Production of a polyclonal antibody against acrylamide for immunochromatographic detection of acrylamide using strip testsLusiani Dewi Assaat0Endang Saepudin1Retno Damayanti Soejoedono2Rahmat Setya Adji3Okti Nadia Poetri4Tribidasari Anggraningrum Ivandini5Department of Chemistry, Faculty of Mathematics and Natural Sciences, Indonesia University, Depok, Indonesia. & Department of Chemistry Education, Faculty of Teacher Training and Education, Sultan Ageng Tirtayasa University, Banten, Indonesia Department of Chemistry, Faculty of Mathematics and Natural Sciences, Indonesia University, Depok, Indonesia Department of Animal Disease and Veterinary Public Health, Faculty of Veterinary Medicine, Bogor Agriculture University, Bogor, Indonesia Center of Veterinary Research, Bogor, Indonesia Department of Animal Disease and Veterinary Public Health, Faculty of Veterinary Medicine, Bogor Agriculture University, Bogor, Indonesia Department of Chemistry, Faculty of Mathematics and Natural Sciences, Indonesia University, Depok, Indonesia.Objective: To produce, purify, and characterize a polyclonal antibody against acrylamide (anti-AA) for an application to immunochromatographic strip tests for AA. Material and Methods: Polyclonal anti-AA was prepared by injecting N-acryloxysuccinimide-conjugated bovine serum albumin hapten-antigen into New Zealand white rabbits. The antibody was purified using protein A, characterized using sodium dodecyl sulfate-polyacrylamide gel elec¬trophoresis (SDS-PAGE) and conjugated with gold nanoparticles (AuNP). The conjugated antibody was then characterized using UVVis and FTIR spectroscopy and transmission electron microscopy (TEM). Immunochromatographic strip tests were performed using sample pads, conjugated pads, test zones, control zones, and absorbent pads. Strip tests were finally validated using standard AA solutions followed by the application of various concentrations of coffee samples. Results: Using SDS-PAGE, the purified anti-AA antibody was resolved at 50 and 25 kDa, indicat¬ing the presence of heavy and light chains, respectively. The conjugation of anti-AA with AuNP was confirmed using wavelength shifts in UVVis and FTIR spectra, and TEM analyses revealed increased diameters of AuNPs after conjugation. The immunochromatographic strip test was sen-sitive to 1 mgml−1 standard AA. Various concentrations of coffee samples resulted in red color differences in the test zone. High and low coffee concentrations produced thick and thin red lines, respectively. Conclusion: Purified anti-AA can be conjugated with AuNP to produce strip tests for detecting AA in coffee samples. The present immunochromatographic strip tests quantitatively showed increasing intensities of red lines with increasing AA concentrations. [J Adv Vet Anim Res 2019; 6(3.000): 366-375]http://www.ejmanager.com/fulltextpdf.php?mno=39101Polyclonal antibody; acrylamide; gold nanoparticles; immunochromatographic strip test; coffee |
collection |
DOAJ |
language |
English |
format |
Article |
sources |
DOAJ |
author |
Lusiani Dewi Assaat Endang Saepudin Retno Damayanti Soejoedono Rahmat Setya Adji Okti Nadia Poetri Tribidasari Anggraningrum Ivandini |
spellingShingle |
Lusiani Dewi Assaat Endang Saepudin Retno Damayanti Soejoedono Rahmat Setya Adji Okti Nadia Poetri Tribidasari Anggraningrum Ivandini Production of a polyclonal antibody against acrylamide for immunochromatographic detection of acrylamide using strip tests Journal of Advanced Veterinary and Animal Research Polyclonal antibody; acrylamide; gold nanoparticles; immunochromatographic strip test; coffee |
author_facet |
Lusiani Dewi Assaat Endang Saepudin Retno Damayanti Soejoedono Rahmat Setya Adji Okti Nadia Poetri Tribidasari Anggraningrum Ivandini |
author_sort |
Lusiani Dewi Assaat |
title |
Production of a polyclonal antibody against acrylamide for immunochromatographic detection of acrylamide using strip tests |
title_short |
Production of a polyclonal antibody against acrylamide for immunochromatographic detection of acrylamide using strip tests |
title_full |
Production of a polyclonal antibody against acrylamide for immunochromatographic detection of acrylamide using strip tests |
title_fullStr |
Production of a polyclonal antibody against acrylamide for immunochromatographic detection of acrylamide using strip tests |
title_full_unstemmed |
Production of a polyclonal antibody against acrylamide for immunochromatographic detection of acrylamide using strip tests |
title_sort |
production of a polyclonal antibody against acrylamide for immunochromatographic detection of acrylamide using strip tests |
publisher |
Network for the Veterinarians of Bangladesh |
series |
Journal of Advanced Veterinary and Animal Research |
issn |
2311-7710 |
publishDate |
2019-09-01 |
description |
Objective: To produce, purify, and characterize a polyclonal antibody against acrylamide (anti-AA) for an application to immunochromatographic strip tests for AA.
Material and Methods: Polyclonal anti-AA was prepared by injecting N-acryloxysuccinimide-conjugated bovine serum albumin hapten-antigen into New Zealand white rabbits. The antibody was purified using protein A, characterized using sodium dodecyl sulfate-polyacrylamide gel elec¬trophoresis (SDS-PAGE) and conjugated with gold nanoparticles (AuNP). The conjugated antibody was then characterized using UVVis and FTIR spectroscopy and transmission electron microscopy (TEM). Immunochromatographic strip tests were performed using sample pads, conjugated pads, test zones, control zones, and absorbent pads. Strip tests were finally validated using standard AA solutions followed by the application of various concentrations of coffee samples.
Results: Using SDS-PAGE, the purified anti-AA antibody was resolved at 50 and 25 kDa, indicat¬ing the presence of heavy and light chains, respectively. The conjugation of anti-AA with AuNP was confirmed using wavelength shifts in UVVis and FTIR spectra, and TEM analyses revealed increased diameters of AuNPs after conjugation. The immunochromatographic strip test was sen-sitive to 1 mgml−1 standard AA. Various concentrations of coffee samples resulted in red color differences in the test zone. High and low coffee concentrations produced thick and thin red lines, respectively.
Conclusion: Purified anti-AA can be conjugated with AuNP to produce strip tests for detecting AA in coffee samples. The present immunochromatographic strip tests quantitatively showed increasing intensities of red lines with increasing AA concentrations. [J Adv Vet Anim Res 2019; 6(3.000): 366-375] |
topic |
Polyclonal antibody; acrylamide; gold nanoparticles; immunochromatographic strip test; coffee |
url |
http://www.ejmanager.com/fulltextpdf.php?mno=39101 |
work_keys_str_mv |
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