MIKUŠOVÁ, Zuzana, Matěj PASTUCHA, Veronika POLÁCHOVÁ, Radka OBOŘILOVÁ, Petr SKLÁDAL and Zdeněk FARKA. Amperometric Immunosensor for Diagnosis of European Foulbrood. In Libuše Trnková. XIX. Workshop of Biophysical Chemists and Electrochemists. 1st edition. Brno: Masaryk University Press, 2019, p. 24-25. ISBN 978-80-210-9309-6.
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Basic information
Original name Amperometric Immunosensor for Diagnosis of European Foulbrood
Authors MIKUŠOVÁ, Zuzana, Matěj PASTUCHA, Veronika POLÁCHOVÁ, Radka OBOŘILOVÁ, Petr SKLÁDAL and Zdeněk FARKA.
Edition 1st edition. Brno, XIX. Workshop of Biophysical Chemists and Electrochemists, p. 24-25, 2 pp. 2019.
Publisher Masaryk University Press
Other information
Original language English
Type of outcome Proceedings paper
Field of Study 10406 Analytical chemistry
Country of publisher Czech Republic
Confidentiality degree is not subject to a state or trade secret
Publication form storage medium (CD, DVD, flash disk)
Organization unit Central European Institute of Technology
ISBN 978-80-210-9309-6
Keywords in English biosensor; amperometry; sandwich assay; antibody; European foulbrood; Apis mellifera
Changed by Changed by: doc. Mgr. Zdeněk Farka, Ph.D., učo 357740. Changed: 20/7/2019 11:36.
Abstract
Western honeybee is an important pollinator and therefore, an invaluable part of agriculture and biodiversity. Serious losses of honeybee colonies in recent years are attributed mostly to climate changes and various diseases. One of the most important microbial diseases of honeybees is European foulbrood (EFB), which is caused by pathogen Melissococcus plutonius. From the economic and environmental point of view, the prevention of EFB spreading is crucial to prevent losses of honeybee colonies. Therefore, the development of an effective method for the detection of M. plutonius is necessary, ideally in the point-of-care (POC) format with sensitivity high enough to detect the pathogen before the clinical symptoms develop. Amperometry and electrochemical impedance spectroscopy (EIS) are highly sensitive and robust approaches compatible with POC testing. Due to their low cost, portability and mass production capabilities, the electrochemical biosensors are typically based on screen-printed electrodes (SPEs). For proper functionality, the immunosensors require antibodies with high affinity and low cross-reactivity. Since there were no antibodies against M. plutonius available, we have prepared them in-house. Purified bacterial cell wall fraction was prepared for rabbit immunization. After 45 days, rabbit blood was collected and serum was prepared. Subsequently, the immunoglobulin G fraction was separated from the serum by liquid chromatography with protein G column. The final antibody in PBS was stored at −30 °C for further use. Functionality of the prepared antibodies was verified using enzyme-linked immunosorbent assay (ELISA). The sandwich assay provided a limit of detection (LOD) of 1.4×10^5 CFU·mL−1. The ELISA was used to detect M. plutonius in real samples of bees, larvae and bottom hive debris, which are the matrices where this bacterium is typically present in the case of EFB infection. For the electrochemical biosensing, the anti-Melissococcus antibody was immobilized on the surface of SPE and allowed specific capture of bacteria. Non-specific binding was evaluated by incubating the sensor with Paenibacillus alvei instead of M. plutonius. The label-free EIS allowed to detect M. plutonius, however, the level of non-specific binding was very high, which was limiting for real samples analysis. Thus, better performance was obtained with amperometric sandwich assay, where the antibodies were conjugated with horseradish peroxidase (HRP). The Ab-HRP conjugate was binding to surface-captured immunocomplex and provided oxidation of 3,3´,5,5´-tetramethylbenzidine (TMB) in presence of H2O2. The electrochemical detection of current was based on the reduction of the enzymatically oxidized TMB on working electrode. For pure bacterial culture in buffer, the LOD was 6.6×10^4 CFU·mL−1. After optimization of amperometric immunosensor, real samples of bees and larvae were tested with LODs 2.4×10^5 CFU·mL−1 and 7.0×10^5 CFU·mL−1, respectively. Time of analysis was only 2 hours compared to time-consuming laboratory assays such as ELISA. The analysis of real bee and larvae samples confirmed the suitability of the developed immunosensor for in-field M. plutonius detection.
Links
LQ1601, research and development projectName: CEITEC 2020 (Acronym: CEITEC2020)
Investor: Ministry of Education, Youth and Sports of the CR
TJ01000386, research and development projectName: Imunostanovení pro diagnostiku hniloby včelího plodu
Investor: Technology Agency of the Czech Republic
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