Fluorescence-based methods for the detection of pressure-induced spore germination and inactivation

被引:12
作者
Baier, Daniel [1 ]
Reineke, Kai [1 ]
Doehner, Isabel [1 ]
Mathys, Alexander [1 ,2 ]
Knorr, Dietrich [1 ]
机构
[1] Tech Univ Berlin, Dept Food Biotechnol & Food Proc Engn, Berlin, Germany
[2] Nestle Res Ctr, CH-1000 Lausanne, Switzerland
关键词
pressure-induced spore germination; flow cytometry; dipicolinic acid; fluorescence-based measurement; BACILLUS-SUBTILIS SPORES; DIPICOLINIC ACID; NUTRIENT;
D O I
10.1080/08957959.2010.527338
中图分类号
O4 [物理学];
学科分类号
0702 ;
摘要
The application of high pressure (HP) provides an opportunity for the non-thermal preservation of high-quality foods, whereas highly resistant bacterial endospores play an important role. It is known that the germination of spores can be initiated by the application of HP. Moreover, the resistance properties of spores are highly dependent on their physiological states, which are passed through during the germination. To distinguish between different physiological states and to detect the amount of germinated spores after HP treatments, two fluorescence-based methods were applied. A flow cytometric method using a double staining with SYTO 16 as an indicator for germination and propidium iodide as an indicator for membrane damage was used to detect different physiological states of the spores. During the first step of germination, the spore-specific dipicolinic acid (DPA) is released [P. Setlow, Spore germination, Curr. Opin. Microbiol. 6 (2003), pp. 550-556]. DPA reacts with added terbium to form a distinctive fluorescent complex. After measuring the fluorescence intensity at 270nm excitation wavelength in a fluorescence spectrophotometer, the amount of germinated spores can be determined. Spores of Bacillus subtilis were treated at pressures from 150 to 600MPa and temperatures from 37 degrees C to 60 degrees C in 0.05M ACES buffer solution (pH 7) for dwell times of up to 2h. During the HP treatments, inactivation up to 2log 10 cycles and thermal sensitive populations up to 4log 10 cycles could be detected by plate counts. With an increasing number of thermal sensitive spores, an increased proportion of spores in germinated states was detected by flow cytometry. Also the released amount of DPA increased during the dwell times. Moreover, a clear pressure-temperature-time-dependency was shown by screening different conditions. The fluorescence-based measurement of the released DPA can provide the opportunity of an online monitoring of the germination of spores under HP inside the HP vessel. Implementation can be done using diamond anvil cells, units with inspection glasses or by inserting an optical fiber into the HP vessel. The analytical methods used can help to understand the complex mechanism of germination and inactivation of bacterial spores. Due to its universal, process-independent character, the application of these methods is feasible for established and emerging technologies.
引用
收藏
页码:110 / 115
页数:6
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