Affiliation:
1. Department of Laboratory Medicine, Mayo Clinic and Mayo Foundation, Rochester, Minnesota 55901
Abstract
Identification of 18 mycobacterial species was performed by analysis of profiles obtained by using gas-liquid chromatography. Organisms were saponified in methanolic NaOH, and the reaction mixture was treated with BF
3
in methanol and extracted with a hexane-chloroform mixture. An identification scheme was developed from 128 stock strains and tested against a collection of 79 clinical isolates. By using gas-liquid chromatographic profiles alone, 58% of specimens were correctly identified to species level, and an additional 41% were correctly identified to a group of two or three organisms. Use in a clinical laboratory over a 2-month period proved chromatography to be as accurate as and more rapid than concurrent biochemical testing. Of 81 isolates tested, 64% were identified to species level by chromatography alone. An additional 35% were differentiated to the same groups of two or three organisms as found in our analysis of stock strains. These groups consisted of:
Mycobacterium tuberculosis, M. bovis
, and
M. xenopi; M. avium
complex,
M. gastri
, and
M. scrofulaceum
; or
M. fortuitum
and
M. chelonei.
Identification to species level from these groups could usually be done by colonial morphology alone and could always be done by the addition of one selected biochemical test. This study demonstrated the practical application of gas-liquid chromatography in the identification of mycobacteria in a clinical laboratory. In particular, all strains of
M. gordonae
and
M. kansasii
were identified to species level.
M. tuberculosis
was definitively identified in 85% of cases. When it could not be definitely identified, the only alternatives were
M. bovis
and
M. xenopi
, both of which are rare causes of infection.
Publisher
American Society for Microbiology
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