Effect of biocides onS. cerevisiae: Relationship between short-term membrane affliction and long-term cell killing
| Autor: | K. Chládková, Tomáš Hendrych, Dana Gášková, P. Goroncy-Bermes, Karel Sigler |
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| Rok vydání: | 2004 |
| Předmět: |
Biocide
Cell Membrane Permeability Protonophore Microbial Sensitivity Tests Saccharomyces cerevisiae Biology Microbiology Membrane Potentials Benzalkonium chloride Anti-Infective Agents medicine Cell damage Fluorescent Dyes Membrane potential Chromatography Cell Membrane Depolarization General Medicine Carbocyanines medicine.disease Spectrometry Fluorescence Cell killing Membrane Biophysics Ethylene Glycols Benzalkonium Compounds medicine.drug |
| Zdroj: | Folia Microbiologica. 49:718-724 |
| ISSN: | 1874-9356 0015-5632 |
| Popis: | The long-term action of recommended (RC) and near-recommended concentrations of several commercial biocides (Lonzabac 12.100, Genamin CS302D, benzalkonium chloride and 2-phenoxyethanol) on cells of S. cerevisiae wild-type strain DTXII was described using plating tests while short-term effects were determined using the potentiometric fluorescent probe diS-C3(3) that detects both changes in membrane potential and impairment of membrane integrity. A 2-d plating of cells exposed to 0.5xRC of benzalkonium chloride and Genamin CS302D for 15 min showed a complete long-term cell killing, with 2-phenoxyethanol the killing was complete only at 2xRC and Lonzabac caused complete killing at RC but not at 0.5xRC. The diS-C3(3) fluorescence assay performed immediately after a 10-min biocide exposure revealed several concentration-dependent modes of action: Lonzabac at 0.5xRC caused a mere depolarization, higher concentrations causing gradually increasing cell damage; benzalkonium chloride and Genamin CS302D rapidly damaged the membrane of some cells and depolarized the rest whereas 2-phenoxyethanol, which had the lowest effect in the plating test, produced a concentration-dependent fraction of cells with impaired membranes. Cell staining slightly increased during the diS-C3(3) assay; addition of a protonophore showed that part of the remaining undamaged cells retained their membrane potential. Comparison of short-term and long-term data implies that membrane depolarization alone is not sufficient for complete long-term killing of yeast cells under the action of a biocide unless it is accompanied by perceptible impairment of membrane integrity. The results show that the diS-C3(3) fluorescence assay, which reflects the short-term effects of a biocide on cell membranes, can be successfully used to assess the microbicidal efficiency of biocides. |
| Databáze: | OpenAIRE |
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