Coupling purification and in situ immobilization process of monoclonal antibodies to clenbuterol for immunosensor application

Coupling purification and in situ immobilization process of monoclonal antibodies to clenbuterol for immunosensor application

Clenbuterol (CL), which promotes the growth of muscular tissue and the reduction of body fat in pigs and cattle, has been confirmed to be a potential hazard to human health. In this study, a monoclonal antibody to clenbuterol (CL mAb) from a hybridoma culture supernatant was purified by an aqueous t...

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Veröffentlicht in:Analytical biochemistry 2015-05, Vol.476, p.59-66
Hauptverfasser: Cao, Hui, Yuan, Min, Wang, Lili, Yu, Jingsong, Xu, Fei
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Sprache:eng
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Animals
Antibodies, Monoclonal - isolation & purification
Aqueous two-phase system
Cattle
Clenbuterol - analysis
Clenbuterol - immunology
Clenbuterol detection
Humans
Immunosensor
In situ immobilization
Monoclonal antibody to clenbuterol
Polyethylene Glycols - chemistry
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creator Cao, Hui
Yuan, Min
Wang, Lili
Yu, Jingsong
Xu, Fei
description Clenbuterol (CL), which promotes the growth of muscular tissue and the reduction of body fat in pigs and cattle, has been confirmed to be a potential hazard to human health. In this study, a monoclonal antibody to clenbuterol (CL mAb) from a hybridoma culture supernatant was purified by an aqueous two-phase system (ATPS) at different polyethylene glycol (PEG) concentrations, PEG molecular weights, pH values, and NaCl concentrations. Then the CL mAb was immobilized in situ by directly adding polystyrene microspheres (PSMSs) into a PEG phase containing CL mAb. Using the immobilized antibody, an immunosensor was constructed to detect the CL residues in pork samples. The results showed that using an ATPS composed of 15% (w/w) PEG6000, 15% (w/w) phosphate, and 15% (w/w) NaCl at pH 8.0, the partition coefficient was 7.24, the activity recovery was 87.86%, and the purification fold was 2.88. The PEG–CL mAb–PSMS retained approximately 98% of its initial activity after 30-ml phosphate buffer (PBS) washings. After 30days of storage, the CL mAb–PSMS lost nearly 75% of its activity, whereas the PEG–CL mAb–PSMS retained as much as 95% of its initial activity. Furthermore, the constructed immunosensor obtained recoveries of 90.5 to 102.6% when applied to pork samples spiked with CL.
doi_str_mv 10.1016/j.ab.2015.01.022
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subjects Animals
Antibodies, Monoclonal - isolation & purification
Aqueous two-phase system
Cattle
Clenbuterol - analysis
Clenbuterol - immunology
Clenbuterol detection
Humans
Immunosensor
In situ immobilization
Monoclonal antibody to clenbuterol
Polyethylene Glycols - chemistry
title Coupling purification and in situ immobilization process of monoclonal antibodies to clenbuterol for immunosensor application
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