One isolate (ECC-Z) was isolated from the Netherlands, and one was isolated in Denmark. Panel B shows the results of a resampling analysis to investigate the probability that the GW 4064 biological activity average phylogenetic distance Necrosulfonamide site between MPEC could be generated by randomly placing MPEC genomes onto the phylogroup A phylogenetic tree. The bell curve in the plot represents the kernel density estimate of 100,000 replications, where the average distance between 66 randomly selected genomes is calculated. The red vertical line represents the actual average distance observed between MPEC. The p-value is calculated by how many of the randomised samples display a distance as low as, or lower, than that observed between MPEC. The distance between MPEC genomes is highly significant (p = 0.00015), indicating that only 15 in 100,000 randomised replications had average distances which were as low or lower than that observed between MPEC genomes. The four vertical grey bars represent the location on the distribution that would yield p-values of 0.0001, 0.001, 0.01, and 0.05, respectively.Scientific RepoRts | 6:30115 | DOI: 10.1038/srepwww.nature.com/scientificreports/communities – a scenario which is unlikely given the diversity of the phylogroup A population. Rather, it is more likely that the overlap in MPEC phylogeny is a result of a similar selective process operating in cattle in each country, which promotes the proliferation of similar lineages of MPEC, presumably based on their inherent gene content. Together, the data summarised in Figs 2 and 3 support previous studies which have shown that the molecular diversity of MPEC may be lower than for other E. coli10,22, and suggests that not all E. coli are equally capable of causing mastitis. This hypothesis has some experimental support, since different E. coli strains vary in their ability to perform functions which may be important for mastitis, such as growth in milk, resistance to phagocytosis, or even fulfilling Koch’s postulates10,21,30. However, although those studies and our data suggest that founder effects are unlikely to play a major role in limiting the diversity of MPEC, further experiments are necessary to ensure that the observed inability for selected strains to cause bovine mastitis extends beyond a deficiency unique to E. coli K7121, for example.Mastitis-associated E. coli possess a larger core genome but a smaller pan-genome than is typical for phylogroup A. Given that the molecular diversity of MPEC is significantly lower than would beexpected from a random selection of phylogroup A isolates, next we investigated the gene content of these organisms to see if the restriction in phylogenetic diversity translated to a restriction of diversity at the gene content level. To do this, we estimated the pan-genome composition of the 533 phylogroup A E. coli, and compared the size of the core genome (genes present in all strains, Fig. 4A) or pan-genome (genes present in any strain, Fig. 4B) between MPEC and the general phylogroup A population. To calculate the curves shown in Fig. 4, we randomly sampled increasing numbers of genomes from both populations over 10,000 replications per data point, where the polygon surrounding the curve represents the standard deviation in the number of genes over the samples. For the analysis of core genes, and because many of the genome sequences used here are in draft form, we permit core genes to be absent in a maximum of one genome of the sample. These data show clearly t.One isolate (ECC-Z) was isolated from the Netherlands, and one was isolated in Denmark. Panel B shows the results of a resampling analysis to investigate the probability that the average phylogenetic distance between MPEC could be generated by randomly placing MPEC genomes onto the phylogroup A phylogenetic tree. The bell curve in the plot represents the kernel density estimate of 100,000 replications, where the average distance between 66 randomly selected genomes is calculated. The red vertical line represents the actual average distance observed between MPEC. The p-value is calculated by how many of the randomised samples display a distance as low as, or lower, than that observed between MPEC. The distance between MPEC genomes is highly significant (p = 0.00015), indicating that only 15 in 100,000 randomised replications had average distances which were as low or lower than that observed between MPEC genomes. The four vertical grey bars represent the location on the distribution that would yield p-values of 0.0001, 0.001, 0.01, and 0.05, respectively.Scientific RepoRts | 6:30115 | DOI: 10.1038/srepwww.nature.com/scientificreports/communities – a scenario which is unlikely given the diversity of the phylogroup A population. Rather, it is more likely that the overlap in MPEC phylogeny is a result of a similar selective process operating in cattle in each country, which promotes the proliferation of similar lineages of MPEC, presumably based on their inherent gene content. Together, the data summarised in Figs 2 and 3 support previous studies which have shown that the molecular diversity of MPEC may be lower than for other E. coli10,22, and suggests that not all E. coli are equally capable of causing mastitis. This hypothesis has some experimental support, since different E. coli strains vary in their ability to perform functions which may be important for mastitis, such as growth in milk, resistance to phagocytosis, or even fulfilling Koch’s postulates10,21,30. However, although those studies and our data suggest that founder effects are unlikely to play a major role in limiting the diversity of MPEC, further experiments are necessary to ensure that the observed inability for selected strains to cause bovine mastitis extends beyond a deficiency unique to E. coli K7121, for example.Mastitis-associated E. coli possess a larger core genome but a smaller pan-genome than is typical for phylogroup A. Given that the molecular diversity of MPEC is significantly lower than would beexpected from a random selection of phylogroup A isolates, next we investigated the gene content of these organisms to see if the restriction in phylogenetic diversity translated to a restriction of diversity at the gene content level. To do this, we estimated the pan-genome composition of the 533 phylogroup A E. coli, and compared the size of the core genome (genes present in all strains, Fig. 4A) or pan-genome (genes present in any strain, Fig. 4B) between MPEC and the general phylogroup A population. To calculate the curves shown in Fig. 4, we randomly sampled increasing numbers of genomes from both populations over 10,000 replications per data point, where the polygon surrounding the curve represents the standard deviation in the number of genes over the samples. For the analysis of core genes, and because many of the genome sequences used here are in draft form, we permit core genes to be absent in a maximum of one genome of the sample. These data show clearly t.