(A) The tachyzoites of T. gondii RH strain infected human 16-HBE cells were fixed with paraformaldehyde and Selleckchem Small molecule library permeablized with Triton X-100. The anti-RhoA and Rac1 primary antibodies were used to bind with the endogenous GTPases, then a FITC conjugated secondary antibody was used to bind with the primary antibodies.
The endogenous RhoA and Rac1 accumulated on the PVM are visualized with a fluorescence microscope. (B-C) COS-7 cells were transfected with 3 μg of pECFP-N1-RhoA-WT and pECFP-N1-Rac1-WT, respectively. Forty-eight hr after transfection, these cells were infected with tachyzoites of T. gondii RH strain (B) or Pru strain (C). Regardless of the virulence of the tachyzoites used for infection, the overexpressed CFP-RhoA and CFP-Rac1 in host cells were recruited to the T. gondii PVM. Bars: 10 μm. Real-time observation of recruitment of RhoA GTPase EVP4593 order to the PVM To follow the events of RhoA GTPase recruitment to the PVM, COS-7 cells transfected with pECFP-RhoA WT were infected with T. gondii
RH tachyzoites. The real-time photographs were taken at 0 min post-infection Ruboxistaurin in vivo and every 5 min thereafter using a confocal fluorescence microscope (Figure 2). Figure 2 The real-time observation of RhoA GTPase being recruited to the parasitophorous vacuole membrane (PVM) following T. gondii tachyzoites invasion (1000×). (A-F) Starting from 0 min after the tachyzoites being added to the COS-7 cells transfected with pECFP-RhoA-WT, the Silibinin invasion of tachyzoites into the host cell was visualized under a confocal microscope and pictures were taken at 5 min intervals. The CFP-tagged RhoA on
the host cell membrane is recruited to the PVM at the same time as the tachyzoites started to invade the host cell (A, pink arrowhead). The accumulation of the RhoA to the PVM continued with the invasion of the tachyzoite into the host cell (B-D, pink arrowhead), until the whole tachyzoite was totally recruited into the host cell (E, white and yellow arrowhead). The loading of the RhoA GTPase onto the PVM continued after the tachyzoite was totally within the host cell, in this case, probably through the means of diffusion from the host cell cytosol (E-H, white and yellow arrowhead). The green fluorescence and the DIC images showing the observation of the invasion processes are provided in Additional file 1: Data S1 and Additional file 2: Data S2. Bar: 10 μm. We found that the CFP-tagged RhoA was recruited to the PVM at the very beginning of the invasion, probably through retention of the RhoA GTPase on the host cell membrane to the PVM, and the accumulation of RhoA on the PVM continued with the recruitment of the tachyzoite until it totally invaded into the host cell (Figure 2A-D: pink arrowhead). However, a focal point of RhoA was not seen at the immediate point of invasion (Figure 2A).