doi: 10.1074/jbc.M110.197111. Epub 2011 Apr 7.
Heterotrimeric Gi proteins link Hedgehog signaling to activation of Rho small GTPases to promote fibroblast migration
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- PMID:21474452
- PMCID: PMC3103338
- DOI: 10.1074/jbc.M110.197111
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Heterotrimeric Gi proteins link Hedgehog signaling to activation of Rho small GTPases to promote fibroblast migration
Ariel H Polizio et al. J Biol Chem..
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Abstract
Evidence supporting the functionality of Smoothened (SMO), an essential transducer in most pathways engaged by Hedgehog (Hh), as a G(i)-coupled receptor contrasts with the lack of an apparently consistent requirement for G(i) in Hh signal transduction. In the present study, we sought to evaluate the role of SMO-G(i) coupling in fibroblast migration induced by Sonic Hedgehog (Shh). Our results demonstrate an absolute requirement for G(i) in Shh-induced fibroblast migration. We found that Shh acutely stimulates the small Rho GTPases Rac1 and RhoA via SMO through a G(i) protein- and PI3K-dependent mechanism, and that these are required for cell migration. These responses were independent of transcription by Gli and of the C-terminal domain of SMO, as we show using a combination of molecular and genetic tools. Our findings provide a mechanistic model for fibroblast migration in response to Shh and underscore the role of SMO-G(i) coupling in non-canonical Hh signaling.
Figures
Shh promotes fibroblast migration through SMO.A, migration of Ptc1+/− mouse embryonic fibroblasts during 8 h after scratching a monolayer in the absence of serum. Vehicle (control) or 2.5 μg/ml Shh were added att = 0 h. Photographs are representative ofn = 6 experiments.B, quantification of Ptc1+/− migration without any stimulus (control), 2.5 μg/ml Shh (Shh), or 5 μm purmorphamine (PUR). Cells were pretreated with DMSO (black bars) or 0.5 μm KAAD-cyclopamine (KAAD) (white bars) (n = 6; *,p < 0.001).C, comparison of spontaneous migration of Ptc1+/− and Ptc1−/− MEFs in the absence or presence of 0.5 μm KAAD.D, quantification of basal Ptc1+/− and Ptc1−/− MEFs migration, the latter in the absence or presence of 0.5 μm KAAD (n = 6; *,p = 0.023). Representative images (E) and quantification (F) of wound healing assays using SMO−/− MEFs treated with 5 μm purmorphamine or 0.5 μm KAAD (n = 6).
SMO-dependent migration requires Gi and PI3K signaling.A, serum-starved Ptc1+/− MEFs were stimulated for 15 min with 5 μm purmorphamine (PUR) or vehicle (control) in the absence or presence of 0.5 μm KAAD-cyclopamine. Whole cell lysates were separated by SDS-PAGE and blotted for P-Akt (Ser-473) and total Akt. Densitometry values of P-Akt (Ser-473) normalized to total Akt represent the mean ± S.E. of three experiments. *,p < 0.05.B, quantification of wound healing assays of Ptc1+/− MEFs pretreated with 100 ng/ml pertussis toxin or 15 μm LY294002 and stimulated with 5 μm purmorphamine or vehicle (DMSO) (n = 6; *,p < 0.001)C–E, representative experiment of P-Akt (Ser-473) and P-PDK1 (Ser-241) levels in serum-starved Ptc1+/− MEFs (C), SMO−/− MEFs (D), and Ptc1−/− MEFs (E) treated overnight with 100 ng/ml PTX or 0.5 μm KAAD-cyclopamine (KAAD) (n = 3).F, migration of Ptc1−/− MEFs (gray bars) or SMO−/− MEFs (black bars) in scratch-wound healing assays (t = 8 h) preincubated with 0.5 μm KAAD-cyclopamine (KAAD), 100 ng/ml PTX, or 15 μm LY294002 (LY). (n = 4–6; *,p < 0.05; ¶,p < 0.01).
Shh stimulates RhoA and Rac1 small GTPases.A, representative Rac1 pulldown assay of serum-starved NIH 3T3 cells stimulated for 0–15 min with 2.5 μg/ml Shh.B, densitometry values of three independent time course Rac1 pulldown experiments. *,p < 0.05.C, representative RhoA pulldown assay of serum starved NIH 3T3 cells stimulated for 0–15 min with 2.5 μg/ml Shh.D, densitometry values of three independent time-course RhoA pulldown experiments; *,p < 0.05; ¶,p < 0.01.E, quantification of wound healing assays of NIH 3T3 cells co-transfected with GFP and pAX142 (empty vector), pAX142-RhoN19, or pAX142-RacN17 and stimulated att = 0 with 2.5 μg/ml Shh or vehicle. Values represent the fold increase of GFP+ cells that migrate into the wound. *,p < 0.05.F, representative images of migration of cells expressing pAX142, pAX142-RhoN19, or pAX142-RacN17 after 8 h in the presence of Shh. Thewhite line shows the scratch border att = 0. Note that green cells expressing pAX142-RhoN19 or pAX142-RacN17 are incapable of moving into the wound.
Constitutive activation of SMO in Ptc1−/− MEFs leads to high basal RhoA and Rac1 activity.A, Ptc1+/− cells were serum-starved for 24 h and stimulated with 2.5 μg/ml Shh or vehicle for 10 min. Ptc1−/− MEFs were serum-starved for 24 h and incubated during the last 45 min with vehicle or 0.5 μm KAAD-cyclopamine. The basal and stimulated levels of GTP-RhoA were determined by pulldown assays as described under “Experimental Procedures.”B, GTP-Rac1 levels were evaluated by pulldown assays in conditions identical toA. Quantification of fractional RhoA (C) and Rac1 (D) GTP loading by densitometry (n = 3; *,p < 0.05).
Shh stimulates RhoA and Rac1 in a SMO-, Gi-, and PI3K-dependent manner.A, representative RhoA pulldown assay of serum starved NIH 3T3 cells stimulated for 10 min with 2.5 μg/ml Shh and pretreated with vehicle, 100 ng/ml PTX, 0.5 μm KAAD-cyclopamine (KAAD), or with 15 μm LY294002.B, representative Rac1 pulldown assay of serum-starved NIH 3T3 cells stimulated for 5 min with 2.5 μg/ml Shh and pretreated as inA. C, densitometry values of three independent RhoA pulldown experiments. *,p < 0.001.D, densitometry values of three independent Rac1 pulldown experiments. *,p < 0.05.
Rac1 activity is required for full RhoA activation by Shh.A, RhoA pulldown assay of Ptc1+/− MEFs transduced with control GFP-AdV or Myc-RacN17-AdV (MOI = 150) and stimulated with 2.5 μg/ml Shh or vehicle (control). Densitometry values of a representative experiment are shownbelow the gel. In thebottom gel, expression of RacN17 was confirmed by Western blot.B, Rac1 pulldown assay of Ptc1+/− MEFs transduced with control GFP-AdV or HA-RhoN19-AdV (MOI = 150) and stimulated with 2.5 μg/ml Shh or vehicle. Densitometry values of a representative experiment are shownbelow the gel. Expression of RhoN19 was confirmed by Western blot to the epitope tag (bottom gel).
Pertussis toxin does not affect Gli-dependent transcription in MEFs.A, expression ofgli1,ptc1, and the housekeeping geneS15 was analyzed by semiquantitative RT-PCR. Ptc1+/− MEFs were grown until fully confluent, pretreated with 100 ng/ml PTX, 0.5 μm KAAD-cyclopamine, or 15 μm LY294002 and then stimulated with 2.5 μg/ml Shh, 5 μm purmorphamine, or vehicle for 24 h in DMEM with 0.5% FBS.B, effect of PTX treatment in Ptc1+/− cells was also quantified by real-time PCR.C, effect of PTX, KAAD-cyclopamine, and LY294002 on the basal expression level ofgli1 in Ptc1−/− and SMO−/− cells.D, expression of Gαz in membranes isolated from Ptc1+/− MEFs or platelets (positive control) by Western blot.
SMO-mediated Rac1 activation is independent of Gli transcriptional activity.A, Ptc1+/− MEFs were transduced with control GFP-AdV or Gli3R-GFP-AdV (MOI = 150). Following 24 h of serum starvation, cells were stimulated with 5 μm purmorphamine (PUR) or vehicle (DMSO) for 5 min, and GTP-Rac1 levels were determined by pulldown assays. Expression of the transgenes was confirmed by Western blot against GFP.B, quantification of GTP-Rac1 activation by purmorphamine in the presence of Gli3R or GFP (n = 3). *,p < 0.05.C, quantification of wound healing assays of Ptc1+/− MEFs transduced with GFP-AdV or Gli3R-GFP-AdV and stimulated att = 0 with 2.5 μg/ml Shh or vehicle. Values represent the fold increase of GFP+ cells that migrate into the wound; *,p < 0.05.D, representative images of migration of cells expressing GFP or Gli3R-GFP after 8 h in the presence of Shh. Thewhite line shows the scratch border att = 0.
SMO promotes monomeric GTPase activation and cell migration independently of its capacity to inducegli1.A,upper gels, expression of SMO variants in membranes prepared from SMO−/− MEFs stably transfected with empty pcDNA3.1vector (pcDNA), SMO-M2 (SMO), SMO-M2-CLD (SMO-CLD), or SMO-M2-ΔC (SMO-ΔC) was assessed by Western blot with anti-SMO E5 mAb. Full-length SMO variants run at ∼90 kDa, whereas SMO-ΔC runs at ∼55 kDa. Theasterisk marks a cross-reactive band.Bottom gels, expression ofgli1 andS15 in the same cell lines was determined by semiquantitative RT-PCR after 24 h of serum starvation at high cell density.B, densitometry values of Rac1 activation of the indicated cell lines after 5 min of stimulation with 5 μm purmorphamine (n = 3; *,p < 0.05; ¶,p < 0.01).C, densitometry values of RhoA activation of the indicated cell lines after 5 min of stimulation with 5 μm purmorphamine (n = 3; *,p < 0.05).D, purmorphamine-induced migration (fold compared with DMSO) of SMO−/− fibroblasts containing empty vector or the three SMO-M2 variants (n = 3). #,p < 0.01; *,p < 0.05.
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