Identification of Mycobacterial Species by Comparative Sequence Analysis of the RNA Polymerase Gene ( rpoB )

Author:

Kim Bum-Joon1,Lee Seung-Hyun1,Lyu Mi-Ae1,Kim Seo-Jeong2,Bai Gill-Han3,Kim Sang-Jae3,Chae Gue-Tae4,Kim Eui-Chong5,Cha Chang-Yong1,Kook Yoon-Hoh1

Affiliation:

1. Department of Microbiology and Cancer Research Center1 and

2. Department of Pediatrics, Pundang CHA General Hospital, Pochun CHA Medical School, Kyonggi-do Sungnam 463-670,2

3. Korean Institute of Tuberculosis, Korean National Tuberculosis Association, Seoul 137-140,3 and

4. Institute of Hansen’s Disease, The Catholic University Medical College, Seoul 137-7014,4 Korea

5. Department of Clinical Pathology,5 Seoul National University College of Medicine, Seoul 110-799,

Abstract

ABSTRACT For the differentiation and identification of mycobacterial species, the rpoB gene, encoding the β subunit of RNA polymerase, was investigated. rpoB DNAs (342 bp) were amplified from 44 reference strains of mycobacteria and clinical isolates (107 strains) by PCR. The nucleotide sequences were directly determined (306 bp) and aligned by using the multiple alignment algorithm in the MegAlign package (DNASTAR) and the MEGA program. A phylogenetic tree was constructed by the neighbor-joining method. Comparative sequence analysis of rpoB DNAs provided the basis for species differentiation within the genus Mycobacterium . Slowly and rapidly growing groups of mycobacteria were clearly separated, and each mycobacterial species was differentiated as a distinct entity in the phylogenetic tree. Pathogenic Mycobacterium kansasii was easily differentiated from nonpathogenic M. gastri ; this differentiation cannot be achieved by using 16S rRNA gene (rDNA) sequences. By being grouped into species-specific clusters with low-level sequence divergence among strains of the same species, all of the clinical isolates could be easily identified. These results suggest that comparative sequence analysis of amplified rpoB DNAs can be used efficiently to identify clinical isolates of mycobacteria in parallel with traditional culture methods and as a supplement to 16S rDNA gene analysis. Furthermore, in the case of M. tuberculosis , rifampin resistance can be simultaneously determined.

Publisher

American Society for Microbiology

Subject

Microbiology (medical)

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