Table 1 The composition of the five simulated clinical samples and the detection of bacteria in each Genome/ Mixture A B C D E   1 2 3 1 2 3 1 2 3 1 2 3 1 2 3 A. baumannii 1.75 1 1   0 0 3.5 1 1 3.5 1 1   0 0 B. fragilis   0 0 1.8 1 1   0 0 1.8 1 1   0 0 B. longum 10.0 1 1   0 0   0 0   0 0   0 0 E. coli 2.25 1 1   0 0   0 0   0 0 0.45 1 1 L. acidophilus 10.0 0 1   0 0   0 0   0 0   0 0 L. brevis   0 0   0 0 10.0 1 1   0 0   0 0 L. gasseri   0 1 10.0 1

1 1.6 1 1   0 0 1.6 1 1 S. aureus   0 0 2.2 1 1   0 0 10.0 1 1   0 0 S. agalactiae   0 0 2.4 1 1   0 0 10.0 1 1   0 0 T. pallidum 0.3 1 1   0 0 3.0 1 1   0 0 10.0 1 1 The five simulated clinical samples are selleck compound labeled A-E. Columns 1: Genomic DNA concentration, ng/μl. SN-38 in vivo Columns 2: Tag4 results. Columns 3: SOLiD results. In columns 2 and 3, “”1″”, a majority of the molecular probes for that genome was positive. “”0″”, a majority of the molecular probes for that genome was not positive Within the Tag4 data, we found one false negative and no false positives. The false negative was for L. acidophilus in simulated clinical sample A (SCA). Two of the four L. acidophilus molecular probes were positive for SCA. Since 50% is not a majority, we could not call L. acidophilus present.

None of the four L. acidophilus molecular probes was positive for any of the other four simulated clinical samples, not even when two other members of the same genus, L. brevis and L. gasseri, were present: that is, there was no cross-reaction. For each of the five simulated clinical samples, we counted a large number of bacteria correctly negative: SCA, 34 correct Sapitinib Cepharanthine negatives; SCB, 35; SCC, 36; SCD, 35, SCE, 36. Taken as a whole, the results for the simulated clinical samples and the two assays (Tag4 and SOLiD) were in excellent qualitative agreement. However,

quantitative agreement between the two methods was not as good. As an example, the SOLiD assay for SCB is shown in Figure 2. (The analogous data for the other four simulated clinical samples are shown in Additional file 1: Figures S1-S4.) The molecular probe leading to the most sequence reads was for Streptococcus agalactiae DNA. This number was dramatically different from the number of sequence reads for the second S. agalactiae probe (Figure 2). The second highest number of sequence reads was for one molecular probe for Bacteroides fragilis DNA. However, B. fragilis DNA was present in the least amount of the four genomic DNAs (Figure 2). Figure 2 Quantitative data for the SOLiD assay for simulated clinical sample B (SCB). The red crosses indicate the known concentrations of each genomic DNA (right ordinate). The horizontal lines indicate the number of sequence reads for each individual molecular probe (left ordinate). Individual bacteria are listed alphabetically across the abscissa.