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. 2009 Nov 16;4(11):e7841. doi: 10.1371/journal.pone.0007841

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Crampton et al.

This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.

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(A) Schematic representation of Dvl1, 2 and 3 showing the proline –rich, putative SH3-binding domains (Proline Rich Regions, or PRR). PRR2 was identified previously in drosophila Dsh as a domain critical for its function. (B) Dvl2 and Grb2 co-immunoprecipitate. FLAG-tagged Dvl2 and HA-tagged Grb2 were expressed individually or together in HEK293 cells. 24 hrs later, the cells (∼5–6×10⁶) were harvested and lysed for 15 min in RIPA buffer containing protease and phosphatase inhibitors. Lysates were cleared, and Dvl2 immunoprecipitated overnight at 4°C with anti-FLAG antibodies. Immune complexes were captured with protein-G coated sepharose beads for 2 hrs at RT. An isotype control antibody was used in parallel. Strips were cut from the same blot and were probed with anti-FLAG or anti-HA antibodies. Whole cell lysate (WCL) was used as a control. (C) Dvl2 and Grb2 co-localize in cells. Confocal microscopy demonstrates punctate distribution of both proteins with considerable cytoplasmic co-localization. Dvl2 is also found in the nucleus. Isotype control staining was negative. (D) Dvl2 and Grb2 synergize to drive LEF/TCF-dependent transcription. HEK293 cells were co-transfected with sTOPflash or the negative control sFOPflash along with GFP, Dvl2, Grb2 or Dvl2 and Grb2 together. Cells were harvested 24 hrs later for luciferase analysis. * – effect of Dvl2 + Grb2 differs significantly from effect of either alone: p<0.01. (E) Dose dependent synergy of Grb2 with Dvl2. HEK293 cells were transfected with sTF as in (D) along with Dvl2 and increasing doses of Grb2. Cells were harvested 24 hrs later. p<0.01 at all time points. (F) The onset of synergy is rapid. HEK293 cells were transfected with GFP, Dvl2, Grb2, or Dvl2 and Grb2 together. Three hrs post recovery was set as t = 0 as this was the earliest GFP could be detected above background. Cells were then harvested at: t = 2,6,10,18 and 24 hrs. Synergy between Dvl2 and Grb2 is achieved as early as 6 hrs (see inset). For all time points 6 hrs and beyond, p<0.01. All luciferase data are normalized to total protein content. Mean and standard error of the mean are shown – where absent, the SEM falls within the symbol. Significance assessed by Student's t-test.