This is probably due to the samples representing

a wider

This is probably due to the samples representing

a wider breadth of the population than the genomes used to calculate the core genome size in previous studies. The remaining 30% of the genome, often known as the accessory genome, is composed of many classes of genes but common themes include those that encode for functions that can mobilise DNA and those that are involved in protein transport/secretion. The former may be responsible for driving a dynamic genome in the species by permitting many mechanisms selleck for horizontal gene transfer. The latter could be involved with niche adaptation. This and other studies have shown that recombination is a significant driver of evolution of the L. pneumophila genome. However we show that the genetic signal contained in the seven loci of the SBT scheme is generally indicative of its genomic heritage. Some STs appear to have been derived from recombination between strains of two different genetic backgrounds. However by clustering STs using BAPs we can determine which STs are likely to exhibit admixture and therefore cannot be confidently assigned to a cluster. Future studies will include looking at strains within and between clusters to determine phenotypes that are shared within a cluster but differ between clusters, and subsequently to search for the genetic

differences that correlate with these phenotypes. Methods For L. pneumophila all STs up to and including ST850 (n = 838 after removing ‘withdrawn’ STs) this website were used in the study. A ST is ‘withdrawn’ when the depositor informs the database curators that the unique allelic profile was submitted in error and

is in fact not extant. As comparator data the following MLST datasets (1 representative per ST) as present in the pubmlst.org data (July 2010 and downloaded from the links present at the URL http://​pubmlst.​org/​data/​) were included; Staphylococcus aureus (clonal), Streptococcus pneumoniae (intermediate) and Neisseria meningitidis (panmictic). Tests for recombination To examine recombination within the L. pneumophila, S. aureus, S. pneumoniae and N. meningitidis populations the following types of events were tested for: Recombination between genes (intergenic) Three methods were used to test for this a. Standardised Index of Association as Implemented Etofibrate in Start 2 [40].   b. Recombination to mutation ratio (r/m) ratio as implemented by ClonalFrame (http://www.xavierdidelot.xtreemhost.com/clonalframe.htm, [41]). The exact method used was as described by Vos et al. [42]. Parameters -x 100000 -y 100000 -z 100 -M -m (where is the Watterson estimate for the scaled mutation rate theta). This is calculated as the number of segregating sites (i.e., the number of polymorphic sites as calculated by DNAsp http://www.ub.edu/dnasp/) divided by the (n-1)th harmonic number where n is the number of samples.

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