The rt-PCR data, but not the microarray analysis, also demonstrat

The rt-PCR data, but not the microarray analysis, also demonstrated a second increase in IL-8 mRNA at 24 h, although with noteworthy variance between experiments. While it is possible that this second surge may be MK-1775 research buy explained by MAPK and/or NF-κB activation, it is unlikely that MAPK or NF-κB signaling explain the initial, powerful IL-8 mRNA peak seen at 3 h. The present study is the first to demonstrate that among more than 38 000 human genes, IL-8 was the single most up-regulated gene by gastric epithelial cells in response to H. pylori exposure in vitro, and it appears feasible that mechanisms

other than MAPK or NF-κB activation may be responsible for this up-regulation. Although histopathological

studies indicate that MOI around 10:1 appear in H. pylori-colonized gastric mucosa, laboratory conditions can never replicate the complex physiology of the human stomach. Much higher MOI have normally been used to study in vitro gastric epithelial cell response to H. pylori colonization, and MOI of 300:1 was our incoulum of choice, as we wanted a sufficient inoculum to induce a biological response from AGS cells, both at the mRNA and protein levels, as indicated by other experiments [35, 63–71]. However, it is worth noting that in a recent report by Ritter et al., a marked IL-8 response from AGS cells exposed to cagA + H. pylori was seen at MOI ranging from 10:1 to 100:1 [61]. The IL-8 QNZ ic50 response was higher at MOI 100:1 compared

enough to 10:1 in all the bacterial strains tested. The response to MOI 300:1 was not assessed. Neither cagA nor vacA status seemed to affect the IL-8 response at the higher inoculum. Ritter’s study also showed that different cellular pathways were activated in response to high or low MOI. In some other studies, where non-gastric cells were exposed to cagA + H. pylori, low MOI was associated with apoptosis inhibition and cell growth, whereas high MOI stimulated apoptosis and inhibited survival [35, 72, 73]. Hence, the choice of MOI may be crucial for the study outcome. Nevertheless, based on our immunofluorescence studies, where we found sufficient bacterial adhesion to AGS cells, typical morphological changes, and most importantly, a marked IL-8 mRNA and protein response to MOI 300:1, we concluded that under our experimental conditions, 300:1 was adequate to elicit a biological response without overloading the system. You et al. performed a similar microarray study published in 2010 [74], where AGS cells were exposed to H. pylori for 6 h. A relatively stable number of Small molecule library chemical structure 300-400 genes were reported to be differentially expressed at each of the sample points, whereas our data showed a progressive increase in the number of genes from 0.5 to 24 h. In addition, key biological processes like chemotaxis, TLR signaling and epithelial cell signaling were reported as down-regulated.

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