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Analysis of survival rates and cellular fatty acid profiles of Listeria monocytogenes treated with supercritical carbon dioxide under the influence of cosolvents

Authors
Kim, Soo RinPark, Hee JungYim, Do SeongKim, Hee TackChoi, In-GeolKim, Young Heon
Issue Date
9월-2008
Publisher
ELSEVIER SCIENCE BV
Keywords
supercritical carbon dioxide; Listeria monocytogenes; food-borne pathogen; inactivation of microorganisms; sterilization
Citation
JOURNAL OF MICROBIOLOGICAL METHODS, v.75, no.1, pp.47 - 54
Indexed
SCIE
SCOPUS
Journal Title
JOURNAL OF MICROBIOLOGICAL METHODS
Volume
75
Number
1
Start Page
47
End Page
54
URI
https://scholar.korea.ac.kr/handle/2021.sw.korea/122809
DOI
10.1016/j.mimet.2008.04.012
ISSN
0167-7012
Abstract
In the present study, we identified several process variables that significantly affect the efficiency of supercritical carbon dioxide inactivation of the food-borne pathogen Listeria monocytogenes. Treatment with SC-CO2 completely disabled the colony-forming activity of the cells (8-log reduction) within specific treatment time (10-50 min), pressure (80-150 bar), and temperature ranges (35-45 degrees C). Microorganism inactivation rates increased proportionally with pressure and temperature, but the inactivation rate decreased significantly when cells were suspended in phosphate-buffered saline rather than in physiological saline. Additionally, when the microbial cell suspension was 80-100% (w/w) of water, the SC-CO2-mediated reduction in CFU ml(-1) was 4-8 log higher at the same treatment conditions than in typical cell suspensions (a water content of 800-4000% [w/w]) or dry preparations that had only 2-10% (w/w) of water. The addition of a fatty acid, oleic acid, decreased the effectiveness of the microbial inactivation by SC-CO2, but the addition of a surfactant, sucrose monolaurate, increased the effectiveness. Therefore, cosolvents for SC-CO2, including water, a fatty acid, and a surfactant in this study, were found to greatly influence on the inactivation effectiveness. The extraction of cellular substances, such as nucleic acid- and protein-like materials and fatty acids, was monitored by spectrophotometry and GC/MS and increased with SC-CO2 treatment time. Additionally, using scanning and transmission electron microscopies, we investigated morphological changes in the SC-CO2-treated cells. The effects of the variables we have described herein represent a significant contribution to our current knowledge of this method of inactivating food-borne pathogens. (C) 2008 Elsevier B.V. All rights reserved.
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