We are first to report the (1) decrease in phagocytosis of mycobacteria by PKC-α deficient macrophages (2) knockdown of PKC-α results in increased survival of mycobacteria within macrophages (3) PknG from Mtb selectively downregulates

PKC-α during infection (4) Expression of PknG in MS reduces the phagocytosis by macrophages and (5) the downregulation of PKC-α is mainly due to the proteolytic degradation by PknG. Results Downregulation of macrophage specific PKC-α by mycobacteria Previous studies suggest that Rv, Ra and BCG are less Inhibitor Library datasheet efficiently taken up by macrophages as compared to MS [19] and have the ability to survive and multiply within macrophages. Infection of Rv but not MS inhibits macrophage PKC-α. The novel (PKC-δ and PKC-θ) and conventional (PKC-ζ) isoforms are not down regulated by Rv Belnacasan solubility dmso infection of macrophages [18]. To know whether infection

Selumetinib of macrophages with BCG and Ra also results in the downregulation of PKC-α, we infected macrophages with mycobacteria and observed that infection of THP-1 cells with BCG and Ra also decreased the expression (2.5 and 5.7 fold respectively) as well as the phosphorylation of PKC-α by 2.5 and 5 fold respectively (Fig. 1A and 1B). Regulation PKC-δ was similar by MS, BCG, Ra and Rv (Fig. 1C) suggesting that pathogenic mycobacteria selectively downregulate PKC-α. The downregulation of PKC-α was also evident in primary mouse peritoneal macrophages when incubated with Rv (Fig. 1D and

1E). Figure 1 Downregulation of PKC-α expression by mycobacteria. THP-1 cells were incubated for 4 h in the presence of mycobacteria (MOI = 1:20) as indicated (C, uninfetced). The cells were lysed, and equal amounts of total cell lysates (20 μg) were resolved by SDS-PAGE and immunoblotted with an antibody against (A) PKC-α and phosphorylated form of PKC-α (Thr638), (B) Densitometric analysis of PKC-α and pPKC-α blots shown in fig. 1A, (C) PKC-δ and phospho-PKCδ Rucaparib price (Thr505). The lower parts of the blots were probed with an anti-tubulin antibody, to assure equal protein loading (lower panel), (D) and (E) level of PKC-α and PKC-δ in mouse peritoneal macrophages. Each experiment was repeated at least 3 times. Decreased phagocytosis and increased survival of BCG and MS within PKC-α deficient THP-1 cells Our initial study has proven that regulation of macrophage PKC-α by mycobacteria is species dependent [18]. To study the effect of PKC-α knockdown on the survival/killing of mycobacteria, THP-1 cells were transfected with SiRNA targeting PKC-α. SiRNA specifically reduced the expression of PKC-α by 70-90% (Fig. 2A). Infection of PKC-α deficient cells resulted in the significant (p < 0.005) reduction in phagocytosis of BCG. Data show that phagocytosis of BCG by PKC-α deficient cells was 2.8 fold reduced when compared to control (Fig. 2B).