COMPARISON OF METHODS FOR OPTIMUM DETECTION OF STRESSED AND LOW-LEVELS OF LISTERIA-MONOCYTOGENES

被引:30
作者
WARBURTON, DW
FARBER, JM
POWELL, C
TIWARI, NP
READ, S
PLANTE, R
BABIUK, T
LAFFEY, P
KAURI, T
MAYERS, P
CHAMPAGNE, MJ
HUNT, T
LACASSE, P
VIET, K
SMANDO, R
COATES, F
机构
[1] AGR CANADA, HLTH ANIM LAB, GUELPH N1G 3W4, ONTARIO, CANADA
[2] COMMUNAUTE URBAINE MONTREAL, SERV ENVIRONM, MONTREAL H4N 2T2, QUEBEC, CANADA
[3] FISHERIES & OCEANS CANADA, FISH INSPECT LAB, BURNABY V5M 4L9, BC, CANADA
[4] HLTH & WELF CANADA, HPB, FOOD STAT & OPERAT PLANNING, OTTAWA K1A 0L2, ONTARIO, CANADA
[5] AGR CANADA, HYG VET LAB, ST HYACINTHE J25 8E3, QUEBEC, CANADA
[6] MANITOBA RES COUNCIL, PORTAGE PRAIRE R1N 3J9, MANITOBA, CANADA
[7] FISHERIES & OCEANS CANADA, FISH INSPECT LAB, St John A1C 5X1, NEWFOUNDLAND, CANADA
[8] ALBERTA DEPT AGR, FOOD LAB, SERV BRANCH, EDMONTON T6H 4P2, ALBERTA, CANADA
[9] MINIST AGR PECHERIES & ALIMENTAT QUEBEC, EXPERTISES & ANAL ALIMENTAIRES LABS, Ste Foy G1P 3W8, QUEBEC, CANADA
[10] NOVA SCOTIA RES FDN, DARTMOUTH B2Y 3Z7, NS, CANADA
[11] FISHERIES & OCEANS CANADA, FISH INSPECT LAB, WINNIPEG R3T 2N6, MANITOBA, CANADA
关键词
D O I
10.1016/0740-0020(92)80020-5
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
Twelve laboratories across Canada participated in this third part of a comparative study of modified versions of the 'FDA' and 'USDA' methods for the detection of Listeria monocytogenes in food and environmental samples. Both methods were modified by the inclusion of additional plating media, as well as by the use of modified Fraser broth in the modified 'FDA' method, and additional 24 h incubation of the enrichment broth in the modified 'USDA' method. Approximately 88-94% of the positive samples were detected after 24 h of enrichment. Incubation of the 'USDA' enrichment broth for 48 h significantly (P<0·05) improved recovery of L. monocytogenes. The modified 'FDA' and 'USDA' methods were comparable (i.e. not significantly different, P>0·05) in their ability to isolate stressed and low levels of L. monocytogenes. The pH of the enrichment broths varied greatly after 24 and 48 h incubation. However, the 'USDA' enrichment broth maintained its pH closer to neutrality which may aid in the isolation of this micro-organism, especially injured cells, from some foods. Modified Fraser broth (MFB) proved to be useful as a secondary enrichment broth, as shown by the significantly greater number (P<0·05) of isolates being recovered from this broth, even though it is not very selective with a 74% false-positive rate. This improved recovery may result from the combination of the use of MFB with the selective plating media. During qualitative testing, Oxford agar (OXA) proved to be the significantly better medium, with lithium chloridephenylethanol-moxalactam medium (LPM), modified Oxford agar (MOX) and Palcam agar (PAL) being comparable in isolating stressed and low levels of this micro- organism from a variety of samples. Quantitative counts of stressed and non-stressed cultures showed that LPM, OXA and PAL were comparable (not significantly different, P>0·05) in their ability to recover stressed cells of this micro-organism. © 1992 Academic Press Limited.
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页码:127 / 145
页数:19
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