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Guide to the Application of Genotyping to Tuberculosis Prevention
and Control
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CDC Tuberculosis Genotyping Laboratory Procedures
Science Behind TB Genotyping
Genotyping is based on an analysis of DNA. Mycobacteria reproduce
by binary fission, which means that in almost all cases each new
bacillus has identical DNA, just as human identical twins are genetically
identical to each other. However, changes in the DNA occur spontaneously
at low frequency. Over time, these changes, known as DNA mutations,
have accumulated to produce the diversity of M. tuberculosis
strains currently circulating in the world.
The diversity of strains provides a means to identify instances
of recent transmission of TB as well as the chains of transmission
that occur among persons with TB. This diversity also helps to elucidate
the patterns and dynamics of TB transmission. When a person with
TB improves but then becomes ill again, this diversity can differentiate
reactivation with the same strain of M. tuberculosis from
reinfection with a different strain. Genotyping can also be used
to identify false-positive cultures.
Advances in DNA analytic methods have made it possible for TB programs
to obtain rapid and reliable genotyping results. These advances
include
- the determination of the complete DNA sequence of M. tuberculosis
in 1998;
- the development of IS6110-based RFLP genotyping, which
provided a discriminatory typing method and led to a standardized
system for genotyping M. tuberculosis isolates; and
- the development of two new methods, spoligotyping and MIRU
analysis, which are based on PCR and provide much more rapid results
than RFLP analysis.
Last Reviewed: 05/18/2008 Content Source: Division of Tuberculosis Elimination
National Center for HIV/AIDS, Viral Hepatitis, STD, and TB Prevention
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