Rapid and Simple Approach for Identification of Mycobacterium tuberculosis Complex Isolates by PCR-Based Genomic Deletion Analysis

doi:10.1128/JCM.40.7.2339-2345.2002

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Journal of Clinical Microbiology, July 2002, p. 2339-2345, Vol. 40, No. 7
0095-1137/02/$04.00+0 DOI: 10.1128/JCM.40.7.2339-2345.2002
Copyright © 2002, American Society for Microbiology. All Rights Reserved.

Rapid and Simple Approach for Identification of Mycobacterium tuberculosis Complex Isolates by PCR-Based Genomic Deletion Analysis

Linda M. Parsons,¹^,2^* Roland Brosch,³ Stewart T. Cole,³ Ákos Somoskövi,¹^,4 Arthur Loder,¹ Gisela Bretzel,⁵ Dick van Soolingen,⁶ Yvonne M. Hale,⁷ and Max Salfinger¹^,2^,8

Wadsworth Center, New York State Department of Health,,¹ Department of Biomedical Sciences, School of Public Health, University at Albany,² Department of Medicine, Albany Medical College, Albany, New York,⁸ Unité de Génétique Moléculaire Bactérienne, Institut Pasteur, Paris, France,³ Department of Respiratory Medicine, School of Medicine, Semmelweis University, Budapest, Hungary,⁴ Bernhard Nocht Institute for Tropical Medicine, Hamburg, Germany,⁵ National Institute of Public Health, Bilthoven, The Netherlands,⁶ Bureau of Laboratories, Florida Department of Health, Jacksonville, Florida⁷

Received 30 January 2002/ Returned for modification 18 March 2002/ Accepted 31 March 2002

Although the virulences and host ranges differ among membersof the Mycobacterium tuberculosis complex (TBC; M. tuberculosis,M. africanum, M. canettii, M. microti, M. bovis, and M. bovisBCG), commercially available molecular assays cannot differentiatethese organisms because of the genetic identities of their 16SrRNA gene sequences. Comparative genomic analyses with the completeDNA sequence of M. tuberculosis H37Rv has provided informationon regions of difference (RD 1 to RD 16) deleted in membersof the TBC other than M. tuberculosis. To determine whetherdeletion analysis could accurately differentiate members ofTBC, we used PCR to assess the presence or absence of specificregions of the genome in 88 well-characterized isolates of M.tuberculosis, M. africanum, M. microti, M. bovis, and M. bovisBCG. The identifications obtained by use of the specific deletionprofiles correlated 100% with the original identifications forall TBC members except M. africanum, but further characterizationresulted in profiles specific for all members. Although sixRD regions were used in the analyses with the original 88 isolates,it was found that the use of RD 1, RD 9, and RD 10 was sufficientfor initial screenings, followed by the use of RD 3, RD 5, andRD 11 if the results for any of the first three regions werenegative. When 605 sequential clinical isolates were screened,578 (96%) were identified as M. tuberculosis, 6 (1%) were identifiedas M. africanum, 8 (1%) were identified as M. bovis, and 13(2%) were identified as M. bovis BCG. Since PCR-based assayscan be implemented in most clinical mycobacteriology laboratories,this approach provides a rapid and simple means for the differentiationof members of TBC, especially M. bovis and M. tuberculosis,when it is important to distinguish between zoonotic sources(i.e., cattle and unpasteurized dairy products) and human sourcesof tuberculosis disease.

* Corresponding author. Mailing address: Wadsworth Center, 120 New Scotland Ave., Albany, NY 12208. Phone: (518) 402-2474. Fax: (518) 474-6964. E-mail: linda.parsons{at}wadsworth.org.

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