001, paired
Student’s t test) ( Figure 1B). On incubation of dihydrorhodamine-1,2,3-loaded monocytes with CRLP (7.5–30 μg cholesterol/ml) there was a rapid increase in ROS formation in comparison to that observed in control cells; after 1 h exposure to CRLP at a dose of 7.5 μg cholesterol/ml there was a 7.5 fold increase selleckchem which was maintained for at least 24 h and was not dose dependent (Figure 2). PDTC, a well-characterised antioxidant with reported ability to inhibit NF-κB activity, reduced both basal and CRLP-induced ROS production (Figure 3A). In contrast, inhibitors of NADPH oxidase (apocynin; PAO; DPI Figure 3C–E) or xanthine oxidase (allopurinol; Figure 3F) had no significant effect on ROS production in CRLP-treated cells. Similarly, neither the MEK inhibitor U0126 (Figure 3B) nor its inactive analogue U0124 (data not shown), affected ROS generation in the presence of CRLP. Freshly isolated human monocytes were incubated with or without CRLP for 6 or 24 h and the secretion of MCP-1 and IL-8 into the medium was measured (n = 5). In the absence of CRLP, the cells secreted high quantities of MCP-1 (CCL2) (5.01 ± 1.58 ng/ml) and IL-8 (CXCL8) (1.54 ± 0.24 ng/ml) after 24 h. Secretion of MCP-1 was decreased by CRLP treatment and this effect was significant after 24 h (6 h, 2.78 ± 0.84 ng/ml; 24 h, 0.65 ± 0.01 ng/ml (P < 0.05)) ( Figure 4A), whilst IL-8 secretion
into the medium was increased ALK inhibitor review Resveratrol at 6 h (3.34 ± 0.30 ng/ml, P < 0.001) and returned to control levels by 24 h (2.77 ± 0.11 ng/ml) ( Figure 4B). Constitutive secretion of both MCP-1 and IL-8 was significantly reduced by treatment with U0126. Production of MCP-1 and IL-8 was also inhibited by PDTC, whereas the NADPH oxidase inhibitor, apocynin, had no effect (Figure 4A, B). Incubation with CRLP did not influence the reduced MCP-1 secretion observed following
treatment with U0126 or PDTC (Figure 4A) but restored IL-8 secretion to constitutive levels in the presence of either inhibitor (Figure 4B.). We hypothesised that the CRLP-driven reduction in MCP-1 secretion may result in increased monocyte chemotaxis due to the resulting increased MCP-1 concentration gradient in the monocyte microenvironment. This was investigated in vitro by testing the migration of cells towards MCP-1 using Transwell chambers ( Figure 5). After pre-exposure to control preparations for 24 h, the number of monocytes migrating to the lower chamber of the Transwells was not significantly different in the presence or absence of MCP-1 in the lower chamber ( Figure 5). Pre-treatment with CRLP, however, caused a significantly higher percentage of monocytes to migrate towards recombinant MCP-1. Addition of recombinant MCP-1 to CRLP-treated monocytes before commencement of the migration assay abolished this effect ( Figure 5). Recent studies have suggested that the interaction of CMR with monocytes may play a part in their atherogenic effects [22], [24] and [27].