Rapid PCR with nested primers for direct detection of Campylobacter jejuni in chicken washes

Rapid detection of Campylobacter jejuni by PCR directly from foods, without prior growth steps, would be beneficial for the poultry industry. We have previously reported a PCR assay that allows detection of this bacterium after 48 h growth on Campy cefex agar. We have now developed a more rapid nest...

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Veröffentlicht in:	Molecular and cellular probes 1997-08, Vol.11 (4), p.267
Hauptverfasser:	Winters, D K, O'Leary, A E, Slavik, M F
Format:	Artikel
Sprache:	eng
Schlagworte:	Agar Animals Base Sequence Campylobacter jejuni - genetics Campylobacter jejuni - isolation & purification Centrifugation Chickens - microbiology DNA Primers - genetics Evaluation Studies as Topic Food Microbiology Meat - microbiology Molecular Sequence Data Polymerase Chain Reaction - methods Sensitivity and Specificity Specimen Handling
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creator	Winters, D K O'Leary, A E Slavik, M F
description	Rapid detection of Campylobacter jejuni by PCR directly from foods, without prior growth steps, would be beneficial for the poultry industry. We have previously reported a PCR assay that allows detection of this bacterium after 48 h growth on Campy cefex agar. We have now developed a more rapid nested PCR assay that specifically detects C. jejuni in chicken washes that have not undergone any lengthy growth steps prior to PCR. For the nested reaction, an external set of primers, C-1 and C-4, are used for 24 cycles. At this time, 1 microl of the PCR product is removed and added to a second reaction. The second PCR assay is run with C-1 and an internal primer, C-2, for 24 cycles. A single band on a 4% NuSieve agarose gel at 122 bp was apparent with C. jejuni cells at a sensitivity of 10(2) cfu ml-1. With this method chicken carcasses can be washed and C. jejuni identified all within 1 day. We detected C. jejuni in approximately 80% of four groups of chickens using this method. The identifications have been confirmed by standard microbiological techniques.
doi_str_mv	10.1006/mcpr.1997.0116
format	Article
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We have previously reported a PCR assay that allows detection of this bacterium after 48 h growth on Campy cefex agar. We have now developed a more rapid nested PCR assay that specifically detects C. jejuni in chicken washes that have not undergone any lengthy growth steps prior to PCR. For the nested reaction, an external set of primers, C-1 and C-4, are used for 24 cycles. At this time, 1 microl of the PCR product is removed and added to a second reaction. The second PCR assay is run with C-1 and an internal primer, C-2, for 24 cycles. A single band on a 4% NuSieve agarose gel at 122 bp was apparent with C. jejuni cells at a sensitivity of 10(2) cfu ml-1. With this method chicken carcasses can be washed and C. jejuni identified all within 1 day. We detected C. jejuni in approximately 80% of four groups of chickens using this method. 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subjects	Agar Animals Base Sequence Campylobacter jejuni - genetics Campylobacter jejuni - isolation & purification Centrifugation Chickens - microbiology DNA Primers - genetics Evaluation Studies as Topic Food Microbiology Meat - microbiology Molecular Sequence Data Polymerase Chain Reaction - methods Sensitivity and Specificity Specimen Handling
title	Rapid PCR with nested primers for direct detection of Campylobacter jejuni in chicken washes
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