Identification of Bordetella pertussis infection by shared-primer PCR.

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J Clin Microbiol. 1994 March; 32(3): 783-789

Identification of Bordetella pertussis infection by shared-primer PCR.

Z Li, D L Jansen, T M Finn, S A Halperin, A Kasina, S P O'Connor, T Aoyama, C R Manclark and M J Brennan

Division of Bacterial Products, U.S. Food and Drug Administration, Bethesda, Maryland 20892.

ABSTRACT

A shared-primer PCR method for the detection of infection wasdeveloped by using primers derived from DNA sequences upstreamof the structural genes for the porin proteins of Bordetellapertussis and Bordetella parapertussis. This method resultedin a 159-bp PCR product specific for B. pertussis and a 121-bpDNA fragment specific for B. parapertussis and allowed for thesimultaneous detection of these pathogens. The PCR procedurewas shown to be very specific since no PCR product was obtainedfrom 36 non-Bordetella bacterial DNAs. Nasopharyngeal aspirates(NPAs) from children suspected of having pertussis were evaluatedby the PCR method, culture, and the Chinese hamster ovary (CHO)cell assay, which detects pertussis toxin. B. pertussis wascultured from 119 of 205 NPAs assayed, and the presence of pertussistoxin was detected in 69 of the NPAs by the CHO cell assay.When ethidium bromide staining was used to detect PCR products,100 NPAs gave positive results by shared-primer PCR; 94 of theseNPAs were also positive by culture. The result indicated a sensitivityof 79% for PCR when culture was used as the standard. The sensitivityof PCR was increased to 95% when a digoxigenin immunoblot systemwas used. An additional 20 NPAs from patients with suspectedpertussis that were culture negative also gave positive resultsby PCR. The specific and sensitive PCR method described hereshould be useful for both the clinical diagnosis of pertussisand case identification in vaccine trials.

J Clin Microbiol. 1994 March; 32(3): 783-789

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