In good agreement with previously published results, we found tha

In good agreement with previously published results, we found that LPS-induced mitochondrial ROS was substantially contributing to the IL-1β production, as shown by the significant (about two-third) inhibition caused by MitoTempo, However, the RWE-mediated enhancement of the IL-1β production does not appear to be as strongly Torin 1 price dependent on mitochondrial ROS because MitoTempo treatment resulted in less than 40% inhibition of IL-1β production. Nevertheless, DPI treatment completely abolished IL-1β production, independently of the stimulating agents (Fig. 2b). This

inhibition pattern suggests that while the majority of the ROS involved in the LPS-induced IL-1β production is mitochondrial, the ROS involved in the RWE-dependent enhancement is cytosolic, generated by pollen-derived NADPH oxidases. To find out whether RWE-enhanced IL-1β production is mediated by NLRP3 inflammasome, we treated THP-1 https://www.selleckchem.com/products/abt-199.html cells with a specific caspase-1 inhibitor. Z-YVAD-FMK significantly reduced the LPS plus RWE-induced IL-1β production, suggesting the involvement of caspase-1 in RWE-enhanced IL-1β production (Fig. 3a). We have also silenced NLRP3 expression using siRNA in THP-1 cells (Fig. 3b,c). Silencing of NLRP3

completely inhibited IL-1β secretion of stimulated THP-1 macrophages (Fig. 3d), indicating that not only the LPS-induced IL-1β production but also its enhancement by RWE are dependent on NLRP3 inflammasome. Priming step of NLRP3 inflammasome function involves the elevated expression of inflammasome components and pro-IL-1β. We sought to determine how RWE and NADPH treatment affect the expression of NLRP3

inflammasome components. We have found that LPS treatment in THP-1 macrophages significantly induced the expression of NLRP3 (Fig. 4a,b) and procaspase-1 (Fig. 4c,d) at both mRNA and protein levels. Whereas RWE in the presence of NADPH did not affect the expression of these molecules, it further enhanced the LPS-induced procaspase-1 expression at both the mRNA and protein levels (Fig. 4c,d). Though an increased transcription of NLRP3 was also observed, this did not result in significant elevation of the protein amount (Fig. 4b). To see whether the elevated Celecoxib level of procaspase-1 is accompanied by increased caspase-1 activity, we detected the processed forms of caspase-1 using immunoblot techniques, furthermore, we also measured the activity of the enzyme in THP-1 cell lysates using a fluorescent substrate. Our results show that LPS treatment significantly induced caspase-1 processing, moreover, in the LPS-primed cells RWE treatment resulted in a further enhancement of the processing of caspase-1 (Fig. 4f). However, we found that while LPS treatment significantly induced caspase-1 enzyme activity (Fig.

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