When a phylotype was defined using a threshold of 97%

When a phylotype was defined using a threshold of 97% PI3K inhibitor nucleotide sequence similarity, 82 to 326 (average 137) phylotypes were found in each mouse (Table 1). Although the gradients of collector’s curves decreased quickly at approximately 1000 sampled sequences, the number of phylotypes was on the increase even at the highest numbers of sequences sampled (Figure 2). The Chao1 estimator of species richness in eight mice ranged from 114 to 470 (average 197), representing about 40% higher numbers than those observed in the present study (Table 1). Due to the known sequencing error of the Roche/454

technology and the possibility of chimeras, it is fair to say that the numbers of phylotypes calculated in this study are overestimates [18]. Trudel et al. [3] identified only 18 species among 671 cultivated bacterial isolates from the oral cavity of BALB/c mice. By applying this website the averaged rarefaction curves of our data sets, 671 sampled sequence reads would correspond to 44 phylotypes. Although the genetic backgrounds of the mice used in these two studies are

different, the species diversity of murine oral microbiota determined by the culture-dependent method is only 41% of that determined by the culture-independent method. Similarly, over 60% of the 141 predominant species detected in the human oral cavity have not been cultivated [19]. Figure 2 Rarefaction analysis performed by the RDP pipeline. Repeated samples of phylotype subsets were used to evaluate whether further sampling would likely identify additional taxa. Interestingly,

the estimated species richness of murine oral bacterial flora is far lower than that of humans reported by Keijser et al. [6]. A direct comparison between the Keijser et al. findings and our results is inappropriate because the human data represented pooled samples from 71 individuals and was based on very short sequence reads (~100 bp). Nevertheless, the relatively low species richness Sorafenib in vivo of murine oral microbiota is expected due to the dominance of a small number of bacterial species. A comparison of oral microbiota from wild-type and TLR2-deficient mice To evaluate the effect of TLR2 deficiency on oral microbiota, the relative abundance of each taxon at the different taxonomic ranks ranging from phylum to species was compared between wild-type and TLR2-deficient animals. The present study has limitation in that the wild-type and TLR2-deficient animals were not subjected to the same environmental conditions during the entire period. Nevertheless, a Selleckchem GDC0449 significant difference in the relative abundance was found at the species level for three species of bacteria: Staphylococcus sciuri, Staphylococcus xylosus, and Enterococcus faecalis (p < 0.05 for all three species, Figure 1B). The diversity of oral microbiota showed a tendency to increase in TLR2-deficient mice, but this finding was not statistically significant (Table 1).

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