Also, preliminary studies using 25 μg of A castellanii-labeled

Also, preliminary studies using 2.5 μg of A. castellanii-labeled cDNA hybridized to the E. coli O157:H7 microarray showed minimal reactivity to E. coli-specific

features (data not shown). This reduced the probability that low-level protozoa RNA contamination could introduce errors into our transcriptional analysis. Also, there was no indication from the Bioanalyzer results selleck chemical that degraded RNAs from dead or dying bacteria were present in the RNA preparations. Statistical analysis indicated that 969 genes with an estimated fold change >1.3 demonstrated transcriptional differences with a P-value<0.018 and an estimated false discovery rate (FDR) of 1.9%. This represents 20% of the genes on the microarray and 17.5% of the genes in the genome and virulence plasmid. Significance and differences in transcript levels for all genes are depicted as a volcano plot seen in Fig. 2. Of the 969 genes differentially expressed, 655 genes were upregulated while 314 genes were downregulated. Differentially expressed genes involved in virulence

are listed in Table 2. Table 3 lists differentially expressed RG7204 manufacturer genes associated with antibiotic resistance, the SOS response, and iron acquisition/metabolism. These genes cover 21COGs, as shown in Fig. 3. All statistically significant genes with P<0.05 are listed in Supporting Information, Table S1. To validate the microarray studies, eight genes were chosen for qRT-PCR analysis, six upregulated Y-27632 research buy and two downregulated. btuD was used for the control as it did not show differential expression in the microarray study. In every case, the qRT-PCR results corroborated the microarray results with respect to direction of differential expression, as shown in Fig. 4. The degree

of transcript difference measured by qRT-PCR was greater than that measured by microarray, as shown previously (Morey et al., 2006). Escherichia coli O157:H7 has adapted to two distinct habitats: the enteric environment of ruminants and the external environment, namely water, soil, and plant surfaces. It comes into contact with protozoa while in both the rumen and external water environments. During passage through the ruminant gastrointestinal tract, a series of environment shifts are encountered, including aerobe to anaerobiosis, protozoal uptake, rumen fluid, and large pH changes, to better prepare this pathogen for colonization of the lower gastrointestinal tract of cattle (Naylor et al., 2003). To better understand this path from a bacterial perspective, we sought to model individual segments starting with the uptake by protozoa. Ideally, this would involve isolation of protozoa from the rumen, but variability in the protozoa species populations, variability between animals, and the lack of protozoa free of internal bacterial, particularly E. coli, presents difficult problems in experimental design and interpretation of microarray data. Because E.

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