Sample preparation and DNA extraction procedures for polymerase chain reaction identification of Listeria monocytogenes in seafoods

被引：47

作者：

Agersborg, A ^{[1
]}

Dahl, R ^{[1
]}

Martinez, I ^{[1
]}

机构：

[1] NORWEGIAN INST FISHERIES & AQUACULTURE, N-9005 TROMSO, NORWAY

来源：

INTERNATIONAL JOURNAL OF FOOD MICROBIOLOGY | 1997年 / 35卷 / 03期

关键词：

Listeria monocytogenes; seafoods; polymerase chain reaction; food safety;

D O I：

10.1016/S0168-1605(97)01245-2

中图分类号：

TS2 [食品工业];

学科分类号：

0832 ;

摘要：

Five grams of seafood products were inoculated with one to 500 viable or 10(9) heat-killed cells of Listeria monocytogenes. The presence of the pathogen was detected by the polymerase chain reaction (PCR) with primers specific for fragments of the lysteriolysin O (hly) gene (two sets) and for the invasion-associated protein (iap) gene (one set). For DNA preparation, boiling, either alone or in combination with lysozyme and proteinase K treatment, was not always sufficient to lyse L. monocytogenes, while treatment with Triton X-100 produced consistently good DNA suitable for amplification. To avoid false-negative and false-positive results, 48 h incubations were necessary and a subculturing step after an initial 24 h incubation greatly improved the results. The primers that amplified regions of the listeriolysin O gene gave clearer and stronger products than primers for the invasion-associated protein gene. Using this method we were able to detect one to five L. monocytogenes cells in 5 g of product in a total of 55 h. (C) 1997 Elsevier Science B.V.

引用

页码：275 / 280

页数：6

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