burgdorferi might involve TLR-2, keeping in mind that the intact bacterium can activate immune responses by TLR-independent mechanisms 31. For example, MyD88 deletion in mice affects immune-mediated pathogen selleck chemicals clearance, while allowing many inflammatory processes to proceed 32, 33. We pre-treated monocytes with a neutralizing monoclonal antibody against TLR-2 (T2.5) and pulsed them with borrelial lipids, leaving blocking antibody
in culture 34. As noted previously in cytokine-activated monocytes 12, the range of CD1a expression on borrelia-activated cells is broad and the histogram is bimodal in nature. T.2.5 reduces the number and mean level of CD1a expression as compared to isotype-matched antibody-treated controls, but some cells retain detectable staining (Fig. 2B and D). For CD1c, the histogram of activated cells shows a single population with a normal Gaussian distribution,
and treatment with anti-TLR-2 blocked expression to levels seen in unactivated cells (Fig. 2D). Thus, live B. burgdorferi and its hydrophobic components selectively increased group 1 but not CD1d protein expression using TLR-2. CD1 cell surface expression might be induced through the NF-κB signaling pathway within a single cell that expresses both TLR-2 and CD1. Alternatively, RO4929097 cell line CD1 might appear through a multi-cell mechanism in which the TLR-2 expressing cells secrete transferable factors. The single cell model is plausible because we found that TLR-2 and group 1 CD1 are co-expressed on myeloid cells (data not shown). On the other hand, a prior study of cellular infection showed that CD1 appeared on individual myeloid cells harboring fluorescent mycobacteria as well as uninfected bystander cells 13. The natural TLR-2 agonists in B. burgdorferi are chemically diverse, but mechanistic studies could more reliably be carried out using a single compound of defined molecular structure. Therefore, we used a synthetic lipopeptide
(triacyl-CSK4) 34. Validation of this TLR-2 agonist showed its ability 3-mercaptopyruvate sulfurtransferase to stimulate group 1 CD1 protein expression on monocytes in a dose-dependent manner (data not shown). Because this and other preliminary studies found concordant upregulation of CD1a, CD1b and CD1c by TLR agonists 13, 17, we measured CD1a as a surrogate for group 1 CD1 proteins 4. Kinetic studies showed that CD1a expression was transiently detected at high densities after 48–72 h after stimulation (Fig. 3A). When triacyl-CSK4 was pulsed onto cells and then washed off, there was a delay of more than 2 days before CD1a proteins appeared at the surface, even though only 10–60 min of exposure to the initial stimulus was sufficient to trigger CD1a expression (Fig. 3B and data not shown). Prior studies have shown that the proximal signaling events involving MyD88, IRAK4, IRAK1, TRAF6, TAK1, IKK and IκB leading to activation are complete within hours 35–40.