Effect of high-pressure processing on reduction of Listeria monocytogenes in packaged Queso Fresco

被引:46
作者
Tomasula, P. M. [1 ]
Renye, J. A. [1 ]
Van Hekken, D. L. [1 ]
Tunick, M. H. [1 ]
Kwoczak, R. [1 ]
Toht, M. [1 ]
Leggett, L. N. [2 ]
Luchansky, J. B. [3 ]
Porto-Fett, A. C. S. [3 ]
Phillips, J. G. [4 ]
机构
[1] ARS, Dairy & Funct Foods Res Unit, USDA, Eastern Reg Res Ctr, Wyndmoor, PA 19038 USA
[2] Smithfield Foods Inc, Smithfield, VA 23430 USA
[3] ARS, Food Safety & Intervent Technol Res Unit, USDA, Eastern Reg Res Ctr, Wyndmoor, PA 19038 USA
[4] ARS, Off Area Director, USDA, Eastern Reg Res Ctr, Wyndmoor, PA 19038 USA
关键词
high-pressure processing; Queso Fresco; Listeria monocytogenes; microbial inactivation; HIGH HYDROSTATIC-PRESSURE; RHEOLOGICAL PROPERTIES; CHEESE; MILK; INACTIVATION; TEMPERATURE; BACTERIA; GROWTH; NISIN; HEAT;
D O I
10.3168/jds.2013-7538
中图分类号
S8 [畜牧、 动物医学、狩猎、蚕、蜂];
学科分类号
0905 ;
摘要
The effect of high-hydrostatic-pressure processing (HPP) on the survival of a 5-strain rifampicin-resistant cocktail of Listeria monocytogenes in Queso Fresco (QF) was evaluated as a postpackaging intervention. Queso Fresco was made using pasteurized, homogenized milk, and was starter-free and not pressed. In phase 1, QF slices (12.7 x 7.6 x 1 cm), weighing from 52 to 66 g, were surface inoculated with L. monocytogenes (ca. 5.0 log(10) cfu/g) and individually double vacuum packaged. The slices were then warmed to either 20 or 40 degrees C and HPP treated at 200, 400, and 600 MPa for hold times of 5, 10, 15, or 20 mm. Treatment at 600 MPa was most effective in reducing L. monocytogenes to below the detection level of 0.91 log(10) cfu/g at all hold times and temperatures. High-hydrostatic-pressure processing at 40 degrees C, 400 MPa, and hold time >= 15 min was effective but resulted in wheying-off and textural changes. In phase 2, L. monocytogenes was inoculated either on the slices (ca. 5.0 log(10) cfu/g; ON) or in the curds (ca. 7.0 log(10) cfu/g; IN) before the cheese block was formed and sliced. The slices were treated at 20 degrees C and 600 MPa at hold times of 3, 10, and 20 mm, and then stored at 4 and 10 degrees C for 60 d. For both treatments, L. monocytogenes became less resistant to pressure as hold time increased, with greater percentages of injured cells at 3 and 10 mm than at 20 min, at which the lethality of the process increased. For the IN treatment, with hold times of 3 and 10 mm, growth of L. monocytogenes increased the first week of storage, but was delayed for 1 wk, with a hold time of 20 min. Longer lag times in growth of L. monocytogenes during storage at 4 degrees C were observed for the ON treatment at hold times of 10 and 20 min, indicating that the IN treatment may have provided a more protective environment with less injury to the cells than the ON treatment. Similarly, HPP treatment for 10 min followed by storage at 4 degrees C was the best method for suppressing the growth of the endogenous microflora with bacterial counts remaining below the level of detection for 2 out of the 3 QF samples for up to 84 d. Lag times in growth were not observed during storage of QF at 10 degrees C. Although HPP reduced L. monocytogenes immediately after processing, a second preservation technique is necessary to control growth of L. monocytogenes during cold storage. However, the results also showed that HPP would be effective for slowing the growth of microorganisms that can shorten the shelf life of QF.
引用
收藏
页码:1281 / 1295
页数:15
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