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Journal of Clinical Microbiology, January 1999, p. 74-80, Vol. 37, No. 1
0095-1137/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
Multicenter Evaluation of the Fully Automated COBAS
AMPLICOR PCR Test for Detection of Chlamydia trachomatis in
Urogenital Specimens
Jean
Vincelette,1,*
Jurjen
Schirm,2
Marc
Bogard,3
Anne-Marie
Bourgault,1
Dirk S.
Luijt,2
Anne
Bianchi,4
Pieter C.
van
Voorst Vader,5
Ann
Butcher,6 and
Maurice
Rosenstraus6
Centre Hospitalier de l'Université de
Montréal, Campus Saint-Luc, Montréal,
Canada1;
Regional Public Health
Laboratory,2 and
Department of
Dermatology, University Hospital,5 Groningen,
The Netherlands;
Unité de Biologie Moléculaire,
Centre Hospitalier de Meaux, Meaux,3 and
Laboratoire de Virologie, Institut Alfred Fournier,
Paris,4 France; and
Roche Molecular
Systems, Branchburg, New Jersey6
Received 26 June 1998/Returned for modification 3 August
1998/Accepted 2 October 1998
The fully automated COBAS AMPLICOR CT/NG test for the detection of
Chlamydia trachomatis was evaluated in a multicenter trial. Test performance was evaluated for 2,014 endocervical swab and 1,278 urine specimens obtained from women and for 373 urethral swab and 254 urine specimens obtained from men. Culture served as the reference
test. Culture-negative, COBAS AMPLICOR-positive specimens that tested
positive in a confirmatory PCR test for an alternative target sequence
within the C. trachomatis major outer membrane protein gene
were resolved as true positives. The overall prevalence of chlamydia
was 4.3% in cervical swabs and 11.0% in urethral swabs from men. When
the results for each specimen type were considered separately, the
resolved sensitivities were 96.5% (83 of 86) for endocervical swab
specimens, 95.1% (39 of 41) for urine specimens from women, 100.0%
(41 of 41) for urethral swab specimens from men, and 94.4% (17 of 18)
for urine specimens from men; the resolved specificities were 99.4%
(1,912 of 1,924) for endocervical swab specimens, 99.8% (1,204 of
1,207) for urine specimens from women, 98.5% (325 of 330) for urethral
swab specimens from men, and 100.0% (236 of 236) for urine specimens
from men. For the subset of patients from whom both swab and urine
specimens were collected, the combined results for both specimen types
were used to identify all infected patients. Using these combined
reslts as criteria, the resolved sensitivities for the COBAS AMPLICOR test were 82.6% (38 of 46) for endocervical swab specimens, 84.4% (38 of 45) for urine specimens from women, 84.2% (16 of 19) for urethral
swab specimens from men, and 89.5% (17 of 19) for urine specimens from
men. In comparison, the sensitivity of culture was only 56.5% (26 of
46) for endocervical specimens and 63.2% (12 of 19) for urethral
specimens from men. The internal control provided in the COBAS AMPLICOR
test revealed that 2.9% of specimens were inhibitory when they were
initially tested. Nevertheless, valid results were obtained for 99.1%
of specimens because 68.7% of the inhibitory specimens were not
inhibitory when a second aliquot of the original sample was tested. Two
additional COBAS AMPLICOR-positive specimens were detected by retesting
inhibitory specimens. The COBAS AMPLICOR CT/NG test for the detection
of C. trachomatis exhibited equally high sensitivities and
specificities with both urogenital swab and urine specimens and, thus,
is well-suited for use in screening.
*
Corresponding author. Mailing address:
Département de Microbiologie Médicale et Infectiologie,
Centre Hospitalier de l'Université de Montréal, Campus
Saint-Luc, 1058 Saint-Denis, Montréal, Québec, Canada H2X
3J4. Phone: (514) 281-2100. Fax: (514) 281-2443. E-mail: vincelej{at}magellan.umontreal.ca.
Journal of Clinical Microbiology, January 1999, p. 74-80, Vol. 37, No. 1
0095-1137/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
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