1. Canonical Insertion-Deletion Markers for Rapid DNA Typing ofFrancisella tularensis
- Author
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Pär Larsson, Malin Granberg, Dimitri Guala, Mats Forsman, Kerstin Svensson, Linda Karlsson, and Anders Johansson
- Subjects
Microbiology (medical) ,indel loci ,Genetic Speciation ,Epidemiology ,DNA fingerprinting ,lcsh:Medicine ,Minisatellite Repeats ,Multiple Loci VNTR Analysis ,molecular epidemiology ,Polymerase Chain Reaction ,Genome ,lcsh:Infectious and parasitic diseases ,VNTR loci ,INDEL Mutation ,Tandem repeat ,Humans ,lcsh:RC109-216 ,Typing ,Francisella tularensis ,Indel ,molecular phylogeny ,Phylogeny ,DNA Primers ,Genetics ,biology ,Research ,lcsh:R ,food and beverages ,Bacteriology ,biology.organism_classification ,Infectious Diseases ,classification ,DNA profiling ,Genome, Bacterial - Abstract
By combining analysis of indel markers with multiple-locus variable-number tandem repeat analysis, individual strains were identified., To develop effective and accurate typing of strains of Francisella tularensis, a potent human pathogen and a putative bioterrorist agent, we combined analysis of insertion-deletion (indel) markers with multiple-locus variable-number tandem repeat analysis (MLVA). From 5 representative F. tularensis genome sequences, 38 indel markers with canonical properties, i.e., capable of sorting strains into major genetic groups, were selected. To avoid markers with a propensity for homoplasy, we used only those indels with 2 allelic variants and devoid of substantial sequence repeats. MLVA included sequences with much diversity in copy number of tandem repeats. The combined procedure allowed subspecies division, delineation of clades A.I and A.II of subspecies tularensis, differentiation of Japanese strains from other strains of subspecies holarctica, and high-resolution strain typing. The procedure uses limited amounts of killed bacterial preparations and, because only 1 single analytic method is needed, is time- and cost-effective.
- Published
- 2007
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