Bars, 20 μm Figure 4 Cadherin distribution in SkMC after 24 h of T. gondii interaction. Confocal Microscopy www.selleckchem.com/products/torin-2.html analysis showing: (A) In 3-day-old
SkMC cultures, after differentiation, myoblasts present intense cadherin labeling at the contact points (arrows). (B and C) In myoblasts after 24 h of interaction with T. gondii (thick arrow), cadherin (thin arrow) becomes disorganized forming aggregates at different sites, around and inside the parasitophorous vacuole (for detail, see inset). (D) Infected myoblasts after 24 h of interaction with T. gondii have little or no Pifithrin-�� cell line labeling for cadherin at points of cell-cell contact (thick arrow). Note that only uninfected cells show strong cadherin expression (thin arrow). Nuclei of cells and parasites labeled with DAPI, in blue. Bars, 20 μm During myogenesis in vitro, myoblasts interact with the surface of myotubes. The dynamics of this interaction induces
the translocation of cadherin from the extremities of myotubes to the Selleck Eltanexor point of cell-cell contact (Figure 5A, B and inset). Labeling for cadherin was observed at the end of infected myotubes, especially at points of contact with uninfected myoblasts, suggesting migration of cadherin to the sites of possible membrane fusion (Figure 5C-E). Figure 5 Cadherin profile in differentiated cultures after 24 h of T. gondii interaction. (A and inset) Mature (arrowhead) and young myotubes in fusion process with myoblasts (arrows) can be observed by phase contrast microscopy. (B and inset) By fluorescence microscopy, cadherin (in green) appears distributed throughout the myotubes, being more concentrated at the cell membrane during adhesion, while mature myotubes alone show more intense labeling at the extremities. (C) Interferential microscopy shows the adhesion of uninfected myoblasts (arrowhead) with a mature infected myotube (thick arrows). (D) Confocal microscopy analysis shows that infected myoblasts do not reveal cadherin labeling Ergoloid and more infected myotubes present weaker cadherin labeling (arrow). Observe
that despite the weak labeling, in infected myotubes cadherin molecules appear to migrate to the point of contact with uninfected myoblasts (arrowhead). (E) Merge. Bars, 20 μm Western blot analysis of cadherin expression in SKMC infected with T. gondii The total cadherin pool was detected using a pan-cadherin-specific antibody, which recognizes the 130 kDa protein [27], since proteins were extracted from 2-3-day-old uninfected cultures (controls) and T. gondii 24 h infected cultures. Quantitative data obtained by densitometric analysis showed that 3-day-old SkMC presented a reduction of only 10% in the synthesis of cadherin when compared to 2-day-old cultures. Regarding the participation of Toxoplasma in the modulation of cadherin synthesis, our data showed a significant decline of cadherin expression after 24 h of T. gondii-SkMC interaction, reaching a 54% reduction.