These cells have diverse functions Selleck MK 8931 within the host including phagocytosis of bacterial, fungal, parasitic and viral pathogens, cytokine and chemokine biosynthesis for inflammatory mediated responses to invading pathogens as well as regulation of cellular metabolic processes including fatty acid metabolism, iron reprocessing and mineral reabsorption [9–11]. In response to certain biological triggers, monocytes or macrophages form multinucleated giant cells (MNGCs), which

involves the fusion of adjacent cells and results in a multinucleated cell with a single cytoplasmic compartment [12]. MNGCs are a well characterized phenotype in tissue granuloma formation in response to bacterial infection, with the most notable being associated with Mycobacterium tuberculosis (Mtb). Using various animal, human, in vitro cell culture and explant tissue models of Mtb infection it has been demonstrated click here that monocytes develop into various MNGC types, which is essential in the confinement of Mtb within infectious granulomas [13–20]. Likewise,

monocyte and macrophage MNGC formation can be induced in vitro using various conditioned mediums containing exogenous cytokines, lectin, phorbol myristate acetate and even select antibodies [21–32]. The most notable cytokines associated with monocyte and macrophage differentiation into MNGCs are Interleukin-4 (IL-4) and Interferon gamma (IFN-γ). However, recent reports have also demonstrated that MNGC formation is dependent on diverse range of cellular proteins including CD36, TREM-2, E-cadherin, CCL2 TPCA-1 cost and Rac1, MMP9, DC-STAMP, E-cadherin and Syk; all of which are involved in intracellular signaling, cell surface communication, proteolysis, chemotaxis and cellular

transcription [28, 33–43]. A unique phenotypic characteristic of Bp infection, in addition to Burkholderia mallei (Bm) and Burkholderia thailandensis (Bt), is the ability to induce host cell Interleukin-3 receptor MNGC formation following cellular uptake, in both tissue culture cells (i.e. murine macrophages) and in primary human cells (patients with active melioidosis) [44–47]. MNGC formation has been demonstrated in both phagocytic and non-phagocytic cells in addition to patient tissue(s) with active melioidosis [46–54]. The importance of Bp-mediated MNGC formation during infection is currently unknown, but it is possible that cell to cell spread via MNGC allows the pathogen to avoid immune surveillance in vivo. The Bp genome encodes a diverse range of specialized protein secretion systems including three type III secretion systems (T3SS) and six type VI secretion systems (T6SS) [1, 55, 56]. Mutation of the Bp T3SS-3, which is homologous to the Shigella Mxi-Spa and Salmonella SPI-1 T3SSs, results in loss of Bp induced MNGC formation, inability of endosomal escape and loss of virulence in animal models of Bp infection [50, 53, 57].