Affiliation:
1. Department of Bacteriology, Swedish Institute for Infectious Disease Control, S-17182 Solna,1
2. Laboratorio Nacional de Saude Publica, Bissau, Guinea-Bissau2
3. Department of Microbiology, Umeå University, 90 187 Umeå,3
4. Department of Bacteriology, Biomedicum, Swedish University for Agricultural Sciences, S-75123 Uppsala, Sweden,4 and
Abstract
ABSTRACT
Two hundred twenty-nine consecutive isolates of
Mycobacterium tuberculosis
complex from patients with pulmonary tuberculosis in Guinea-Bissau, which is located in West Africa, were analyzed for clonal origin by biochemical typing and DNA fingerprinting. By using four biochemical tests (resistance to thiophene-2-carboxylic acid hydrazide, niacin production, nitrate reductase test, and pyrazinamidase test), the isolates could be assigned to five different biovars. The characteristics of four strains conformed fully with the biochemical criteria for
M. bovis
, while those of 85 isolates agreed with the biochemical criteria for
M. tuberculosis
. The remaining 140 isolates could be allocated into one of three biovars (biovars 2 to 4) representing a spectrum between the classical bovine (biovar 1) and human (biovar 5) tubercle bacilli. By using two genotyping methods, restriction fragment length polymorphism analysis with IS
6110
(IS
6110
RFLP analysis) and spoligotyping, the isolates could be separated into three groups (groups A to C) of the
M. tuberculosis
complex. Group A (
n
= 95), which contained the majority of classical human
M. tuberculosis
isolates, had large numbers of copies of IS
6110
elements (mean number of copies, 9) and a distinctive spoligotyping pattern that lacked spacers 33 to 36. Isolates of the major group, group B (
n
= 119), had fewer IS
6110
copies (mean copy number, 5) and a spoligotyping pattern that lacked spacers 7 to 9 and 39 and mainly comprised isolates of biovars 1 to 4. Group C isolates (
n
= 15) had one to three IS
6110
copies, had a spoligotyping pattern that lacked spacers 29 to 34, and represented biovar 3 to 5 isolates. Four isolates whose biochemical characteristics conformed with those of
M. bovis
clustered with the group B isolates and had spoligotype patterns that differed from those previously reported for
M. bovis
, in that they possessed spacers 40 to 43. Interestingly, isolates of group B and, to a certain extent, also isolates of group C showed a high degree of variability in biochemical traits, despite genotypic identity in terms of IS
6110
RFLP and spoligotype patterns. We hypothesize that isolates of groups B and C have their evolutionary origin in West Africa, while group A isolates are of European descent.
Publisher
American Society for Microbiology
Cited by
72 articles.
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