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Synergism between Hedgehog-GLI and EGFR Signaling in Hedgehog-Responsive Human Medulloblastoma Cells Induces Downregulation of Canonical Hedgehog-Target Genes and Stabilized Expression of GLI1

PLoS ONE (2013) 8(6)
DOI: 10.1371/journal.pone.0065403
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Abstract

Aberrant activation of Hedgehog (HH) signaling has been identified as a key etiologic factor in many human malignancies. Signal strength, target gene specificity, and oncogenic activity of HH signaling depend profoundly on interactions with other pathways, such as epidermal growth factor receptor-mediated signaling, which has been shown to cooperate with HH/GLI in basal cell carcinoma and pancreatic cancer. Our experimental data demonstrated that the Daoy human medulloblastoma cell line possesses a fully inducible endogenous HH pathway. Treatment of Daoy cells with Sonic HH or Smoothened agonist induced expression of GLI1 protein and simultaneously prevented the processing of GLI3 to its repressor form. To study interactions between HH- and EGF-induced signaling in greater detail, time-resolved measurements were carried out and analyzed at the transcriptomic and proteomic levels. The Daoy cells responded to the HH/EGF co-treatment by downregulating GLI1, PTCH, and HHIP at the transcript level; this was also observed when Amphiregulin (AREG) was used instead of EGF. We identified a novel crosstalk mechanism whereby EGFR signaling silences proteins acting as negative regulators of HH signaling, as AKT- and ERK-signaling independent process. EGFR/HH signaling maintained high GLI1 protein levels which contrasted the GLI1 downregulation on the transcript level. Conversely, a high-level synergism was also observed, due to a strong and significant upregulation of numerous canonical EGF-targets with putative tumor-promoting properties such as MMP7, VEGFA, and IL-8. In conclusion, synergistic effects between EGFR and HH signaling can selectively induce a switch from a canonical HH/GLI profile to a modulated specific target gene profile. This suggests that there are more wide-spread, yet context-dependent interactions, between HH/GLI and growth factor receptor signaling in human malignancies. © 2013 Götschel et al.

Figures

  • Figure 1. Daoy cells respond to SAG and Shh-N by upregulating canonical HH/GLI targets. (A) Incubation with SAG (100 nM) induced the expression of GLI1 protein and inhibited processing of endogenous GLI3 to its repressor form. Co-incubation with Cyclopamine (cyc, 5 mM) inhibited the SAG-induced GLI1 expression and promoted processing of GLI3 to its repressor (GLI3R) form and inhibited GLI2 expression. Beta-actin shown as Western blot loading control. (B) Transcripts for GLI1 and PTCH were upregulated after stimulation with Shh-N for 24 h, induction of HHIP transcripts was seen after 48 h. Enhanced GLI1, HHIP, and PTCH expression levels were still observed after 72 hours. (C) Schematic presentation of canonical Hedgehog signaling. Left panel illustrates silencing of Hedgehog-mediated signaling via a PTCH-mediated block of SMO so that repressor GLI3 prevails and limits the expression rate of Hedgehog target genes. The right panel illustrates the ‘‘Hedgehog-on’’ state, activating GLI proteins now control the expression of Hedgehog-target genes such as GLI1, PTCH, and HHIP. Upregulation of PTCH and HHIP will eventually result in the downregulation of Hedgehog-signaling. Red color indicates a protein with inactivating properties, white color indicates a protein with activating properties, and grey color indicates RNA transcripts. doi:10.1371/journal.pone.0065403.g001
  • Figure 2. Uptake of EGF by Daoy cells and time-resolved analysis of EGF- downstream signaling. (A) To measure the EGF receptor binding and depletion of the growth factor from the medium supernatant a fluorescent ELISA was performed. Daoy cells were treated with 5 ng/ml of recombinant EGF, and medium supernatants were collected after the indicated time periods (light grey symbols). To control that the ligand is bound and taken up by the cells, and not just degraded by the incubation conditions within the cell culture incubator, wells without cells served as controls (dark grey symbols). (B) Activation of EGF downstream pathways (PI3K/AKT and MAPK) was analyzed by Western blot with phospho-specific antibodies against AKT and ERK. Prior to the application of 5 ng/ml EGF ligand the cells had been starved in low serum (0.5% FBS) medium o/n to minimize basal pathway activation. After the addition of EGF cell lysates were prepared at the indicated timepoints. One sample remained untreated and served as control. Loading of equal protein amounts was checked by probing the Western blot membranes with ß-Tubulin. doi:10.1371/journal.pone.0065403.g002
  • Table 1. Targets differentially regulated in response to ShhN/EGF-crosstalk.
  • Figure 3. Stimulation of Hedgehog-primed Daoy cells with EGF induced downregulation of canonical HH/GLI targets. Daoy cells were either treated with control medium (purple), Shh-N conditioned medium (blue), EGF (red) or a combinatorial treatment with Shh-N medium and EGF (green) treated for 24 h. (A) Transcript dynamics for GLI1, PTCH, and HHIP were analyzed by transcript profiling on whole genome arrays. Curves represent mean values of independent biological experiments (n = 3, +/2SEM). (B) Taqman RT-PCR confirmed downregulation of canonical Hedghog targets by EGF. doi:10.1371/journal.pone.0065403.g003
  • Figure 4. Downregulation of GLI1 as canonical Hedgehoginduced transcript was not rescued after inhibition of MEK/ERK and PI3K/AKT signaling. (A) Impact of PI3K inhibition using LY294002 on the EGF-induced downregulation of GLI1 transcripts after stimulation of Shh-N primed cells for 3 h with EGFR ligands. (B) Impact of MEK1 inhibition using PD98059 on the EGF-induced downregulation of GLI1 transcripts measured 3 h after ligand stimulation of Shh-N primed cells. Figure S3 shows data from a corresponding experiment using U0126 an inhibitor of MEK1/2 and PI103 as a PI3K inhibitor. doi:10.1371/journal.pone.0065403.g004
  • Figure 5. EGF stimulation of Hedgehog-primed Daoy cells strongly upregulated canonical EGF target genes. Cells were treated with either control medium (purple), Shh-N conditioned medium (blue), EGF (red) or a combinatorial treatment with Shh-N medium and EGF (green). (A) Gene expression profiling data indicated upregulation of MMP7, VEGFA, and IL-8. (B) Taqman Real Time PCR confirmed upregulation of canonical EGF targets in Hedgehog-primed cells. (C) MMP7, VEGFA, and IL-8 protein levels were quantified by ELISA in cell culture supernatants at indicated time points. Average fold-changes or concentrations were obtained as mean of three independent biological experiments (+/2SEM). doi:10.1371/journal.pone.0065403.g005
  • Figure 6. Hedgehog/EGF crosstalk results in maintenance of high GLI1 levels without affecting GLI3 processing. Samples were obtained after inducing EGFR signaling in Shh-N primed Daoy cells (Shh-N) or unprimed Daoy cells (EGF) for 3 h or 18 h with EGF (A) or AREG (B). Control cells were neither primed with SAG nor exposed to EGF. Western blots were probed with antibodies against GLI1, GLI3 and HSP70. Figure S6 A shows GLI3A/GLI3R ratios for crosstalk induced by EGF and AREG. doi:10.1371/journal.pone.0065403.g006
  • Figure 7. Hedgehog/EGF crosstalk analyzed on the signaling level by RPPA. Samples were obtained at 14 time points after inducing EGFR signaling in Shh-N primed Daoy cells or control Daoy cells by EGF. Daoy cells were either treated with control medium (purple), Shh-N conditioned medium (blue), EGF (red) or a combinatorial treatment with Shh-N medium and EGF (green) treated for 24 h. Data for selected phosphoproteins are shown for short time signaling (A: 0–6 h) and long term signaling (B: 6–24 h). Certain kinases, e.g. MEK and ERK1/2, clearly depend on fast signals mediated by EGFR, most proteins assessed by RPPA show no significant changes on the phosphoprotein level as shown here for p70S6K and GSK3 signaling. Table 2 summarizes phosphoproteins probed by RPPA. doi:10.1371/journal.pone.0065403.g007

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Götschel, F., Berg, D., Gruber, W., Bender, C., Eberl, M., Friedel, M., … Korf, U. (2013). Synergism between Hedgehog-GLI and EGFR Signaling in Hedgehog-Responsive Human Medulloblastoma Cells Induces Downregulation of Canonical Hedgehog-Target Genes and Stabilized Expression of GLI1. PLoS ONE, 8(6). https://doi.org/10.1371/journal.pone.0065403

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