Abstract

Analyses of food-borne pathogens are of great importance in order to minimize the risk of infection for customers. These analyses should be as fast as possible. Any detection method requires enrichment and quantitative analysis of the enriched microbes. Conventional enrichment methods, which take several days, need to be replaced by faster techniques such as biomagnetic separation (BMS). This technique involves the use of paramagnetic microspheres coated with ligands that have special affinity to the microbes that have to be detected. In the studies reported here, enrichment experiments by BMS were carried out using the non-pathogenic E. coli DSM 498 as a model strain and beads coated with a polyethylenimine (PEI) anion-exchange material. The results show that the number of cells separated, as a proportion of the total, was positively correlated with the bead concentration and the length of the period they were mixed together. In addition, a mathematical model, based on the rate of impact between two different sorts of particles, was developed to describe the proportion of separated cells as a function of incubation time and the concentration, size and density of the beads and cells. This is the first mathematical description of cell-bead interactions to be based on well-understood physicochemical principles. The model was confirmed by separation experiments in which the concentration of beads and the incubation period were varied. The developed model enables optimization of the amount of beads added and the reaction period necessary for complete cell separation and thus minimization of costs in BMS.

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