Reliability of Nested PCR for Detection of Chlamydia pneumoniae DNA in Atheromas: Results from a Multicenter Study Applying Standardized Protocols

doi:10.1128/JCM.40.12.4428-4434.2002

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Journal of Clinical Microbiology, December 2002, p. 4428-4434, Vol. 40, No. 12
0095-1137/02/$04.00+0 DOI: 10.1128/JCM.40.12.4428-4434.2002
Copyright © 2002, American Society for Microbiology. All Rights Reserved.

Reliability of Nested PCR for Detection of Chlamydia pneumoniae DNA in Atheromas: Results from a Multicenter Study Applying Standardized Protocols

Petra Apfalter,¹^* Ojan Assadian,² Francesco Blasi,³ Jens Boman,⁴ Charlotte A. Gaydos,⁵ Michael Kundi,⁶ Athanasios Makristathis,¹ Marion Nehr,¹ Manfred L. Rotter,¹ and Alexander M. Hirschl¹

Division of Clinical Microbiology,¹ Division of Hospital Hygiene, Hygiene-Institute,² Department of Occupational and Social Hygiene, Institute of Environmental Health, University of Vienna, Vienna, Austria,⁶ Institute of Respiratory Diseases, University of Milan, IRCCS Policlinico, Milan, Italy,³ Department of Clinical Virology, Umeå University Hospital, Umeå, Sweden,⁴ Department of Medicine, Division of Infectious Diseases, The Johns Hopkins University, Baltimore, Maryland⁵

Received 7 March 2002/ Returned for modification 13 July 2002/ Accepted 12 August 2002

The present multicenter study was designed to find explanationsfor the discrepancies in the reported rates of detection ofChlamydia pneumoniae DNA in endarterectomy specimens. Codedidentical sets of (i) a C. pneumoniae DNA dilution series (panel1; n = 10), (ii) spiked control tissue specimens (panel 2; n= 10 specimens, including 5 negative controls), and (iii) endarterectomyspecimens (panel 3; 15 atheromas, 5 negative controls) wereanalyzed at four laboratories by three standardized DNA extractionmethods in each laboratory and a nested touchdown PCR protocoltargeting the ompA gene of C. pneumoniae. Panel 1 samples werecorrectly identified as positive to levels of 0.3 inclusion-formingunits (IFU)/PCR mixture (100%) and 0.03 IFU/PCR mixture (50%).All negative controls were correctly reported as negative. Panel2 samples were identified as C. pneumoniae positive to levelsof 0.01 IFU/PCR mixture (100%) and 0.005 IFU/PCR mixture (91%),independent of the DNA extraction method used, and only onefalse-positive result was reported. For panel 3 samples, 5 of240 (2%) analyses (in which DNA extractions and PCR were performedat the same laboratory) were positive; the positive specimenswere from three endarterectomy specimens and two negative controls.After exchange of DNA extracts between laboratories, 13 of 15atheroma samples were C. pneumoniae DNA positive in at least1 of a series of 48 analyses per atheroma sample; however, theoverall positivity rate did not exceed 5% (33 of 720 analyses)and therefore was lower than that for the negative controls(8%; 19 of 240 analyses). Not a single positive result couldbe achieved when all panel 3 extracts (n = 240 analyses) werereamplified by a 16S rRNA PCR followed by hybridization witha C. pneumoniae-specific probe. Statistical analyses demonstratedthat positive results did not occur in an independent and randomfashion and could most likely be explained by amplicon carryoverat the nested PCR level as well as amplicon introduction duringDNA extraction, but not by the patterns of distribution of verylow target levels or a certain DNA extraction protocol. Theresults of studies by nested PCR for detection of the prevalenceof C. pneumoniae will always be questionable.

* Corresponding author. Mailing address: Department of Clinical Microbiology, Hygiene-Institute, University of Vienna, Vienna University Hospital, Währinger Gürtel 18-20/5P, A-1090 Vienna, Austria, Phone: 43 (1) 40400-5151. Fax: 43 (1) 40400-5228. E-mail: Petra.Apfalter{at}akh-wien.ac.at.

Journal of Clinical Microbiology, December 2002, p. 4428-4434, Vol. 40, No. 12
0095-1137/02/$04.00+0 DOI: 10.1128/JCM.40.12.4428-4434.2002
Copyright © 2002, American Society for Microbiology. All Rights Reserved.

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