A majority of the proteins in this data set are predicted to reside in the cytoplasm (14 proteins) and cell nucleus (9 proteins). Six proteins are predicted to function in the extracellular space while four proteins are thought to be located on the plasma membrane. Other than cellular location, the host genes were also categorized on the

basis of the expressed protein’s function – i.e. enzyme, cytokine, transporter, transcriptional regulator, or other. For the thirty-six gene subset, Table 1 also lists the fold change found within the separate mock treated and CAM treated microarrays, respectively, as well as the fold difference between the arrays. C. burnetii infected host cells had lower RNA levels of twenty-two host genes relative to cells containing C. burnetii transiently inhibited EPZ004777 nmr with CAM. RNA levels of fourteen genes in this data set are found to be higher due to C. burnetii infection when compared to the CAM treated condition. Bioinformatic analysis conducted to determine possible biological functions of these C. burnetii modulated

host genes indicates that immune response and cellular movement, cellular signaling, cellular proliferation, cell death, lipid metabolism, molecular transport, as well as vesicle trafficking, and cytoskeletal organization are affected by C. burnetii protein synthesis (Table 1). These data indicate that the click here expression of vital genes involved in cellular movement – IL8, CCL2, CXCL1, SPP1 (cytokines) are suppressed via C. burnetii’s protein synthesis in mock treated conditions when compared to CAM

find more treated conditions. These secretory molecules (IL8, CCL2, CXCL1, SPP1) regulate the infiltration and trafficking of immune cells. Table 1 shows other crucial host Amylase genes specifically suppressed by C. burnetii protein synthesis in THP-1 infection such as BCL3, CTSB and CTSL1 (apoptosis), MTSS1, SMTN and PLEKHO1 (cytoskeleton organization), APOE, PLIN2 and FABP4 (lipid metabolism), and RAB20, SOD2, PSMA8, MSC, ZFP36L1, and RORA (Miscellaneous). The prominent genes found to be up-regulated (induced) due to C. burnetii’s protein synthesis are ITK, DUSP9 & SKP2 (intracellular signaling), SOX11, HELLS & PGR (cell growth and proliferation) SLC22A6, CDH2, PSD4, ZNF573, CHMP5 & MRPL44 (Miscellaneous) and ANLN (cytoskeleton organization). Table 1 Differentially expressed host genes modulated by C. burnetii protein synthesis. Cellular Function Gene Symbol Cellular location Predicted Function(s) -CAM1 +CAM2 FD3   CTSB Cytoplasm peptidase 3.102 6.565 ↑3.463 Apoptosis CTSL1 Cytoplasm peptidase 3.173 6.914 ↑3.741   BCL3 Nucleus transcription regulator 3.103 5.673 ↑2.57   C11ORF82 Cytoplasm other -1.849 -4.912 ↓3.062 Cell proliferation SOX11 Nucleus transcription regulator 3.127 -2.915 ↓6.042   HELLS Nucleus enzyme -1.551 -4.653 ↓3.101   PGR Nucleus ligand-depend. nuclear recept. -1.539 -6.853 ↓5.