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Regulation of Constitutive GPR3 Signaling and Surface Localization by GRK2 and β-arrestin-2 Overexpression in HEK293 Cells

PLoS ONE (2013) 8(6)
DOI: 10.1371/journal.pone.0065365
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Abstract

G protein-coupled receptor 3 (GPR3) is a constitutively active receptor that maintains high 3′-5′-cyclic adenosine monophosphate (cAMP) levels required for meiotic arrest in oocytes and CNS function. Ligand-activated G protein-coupled receptors (GPCRs) signal at the cell surface and are silenced by phosphorylation and β-arrestin recruitment upon endocytosis. Some GPCRs can also signal from endosomes following internalization. Little is known about the localization, signaling, and regulation of constitutively active GPCRs. We demonstrate herein that exogenously-expressed GPR3 localizes to the cell membrane and undergoes internalization in HEK293 cells. Inhibition of endocytosis increased cell surface-localized GPR3 and cAMP levels while overexpression of GPCR-Kinase 2 (GRK2) and β-arrestin-2 decreased cell surface-localized GPR3 and cAMP levels. GRK2 by itself is sufficient to decrease cAMP production but both GRK2 and β-arrestin-2 are required to decrease cell surface GPR3. GRK2 regulates GPR3 independently of its kinase activity since a kinase inactive GRK2-K220R mutant significantly decreased cAMP levels. However, GRK2-K220R and β-arrestin-2 do not diminish cell surface GPR3, suggesting that phosphorylation is required to induce GPR3 internalization. To understand which residues are targeted for desensitization, we mutated potential phosphorylation sites in the third intracellular loop and C-terminus and examined the effect on cAMP and receptor surface localization. Mutation of residues in the third intracellular loop dramatically increased cAMP levels whereas mutation of residues in the C-terminus produced cAMP levels comparable to GPR3 wild type. Interestingly, both mutations significantly reduced cell surface expression of GPR3. These results demonstrate that GPR3 signals at the plasma membrane and can be silenced by GRK2/β-arrestin overexpression. These results also strongly implicate the serine and/or threonine residues in the third intracellular loop in the regulation of GPR3 activity. © 2013 Lowther et al.

Figures

  • Table 1. Primer sets used for GPR3-HA mutagenesis.
  • Figure 1. GPR3 is present at the cell surface and undergoes internalization. HEK293 cells were transfected with GPR3-HA. Twentyfour hr later, surface proteins were biotinylated at 4uC (lane 1), allowed to internalize for 30 min (lane 3) or 60 min (lane 4) at 37uC, and biotinylated proteins remaining at the cell surface were removed using a glutathione strip buffer. Biotinylated proteins were precipitated from the total lysate and 5 ml of the sample was analyzed by Western blotting. Lane 2 shows efficient stripping of biotin from the cell surface GPR3. Detection of GAPDH in 0.5 mg of total lysate was run on the same gel and served as a loading control to confirm that an equivalent amount of protein was used for precipitations. Representative blot of 2 separate experiments. doi:10.1371/journal.pone.0065365.g001
  • Figure 2. Inhibition of endocytosis increases cell surface GPR3. (A and B) HEK293 cells were transfected with Dyn WT (A) or Dyn K44A (B) and 24 hr later, the cells were incubated with Alexa Fluor 488-labelled transferrin and imaged with a confocal microscope. Images are representative of 3 separate experiments. (C–E) Cells were co-transfected with GPR3-RFP and pcDNA (C), or Dyn WT (D) or Dyn K44A (E) and imaged using a confocal microscope 24 hr later. Bar = 10 mm. (F) One mg of HEK293 lysate was used to detect Dyn WT and Dyn K44A overexpression by Western blot. (G) HEK293 cells were co-transfected with GPR3-HA and Dyn WT or Dyn K44A and 24 hr after transfection cell surface proteins were biotinylated, precipitated, and surface expression of GPR3-HA was detected by Western blot analysis. 0.5 mg of total lysate was used to detect total GPR3 and GAPDH expression. Blot is representative of 3 separate experiments. (H–I) Bands corresponding to surface GPR3 and total GPR3 expression were analyzed using densitometry. H) Densitometric values for total GPR3 expression in cell lysates were normalized to GAPDH. I) The densitometric value for surface GPR3 was divided by the densitometric value for total GPR3 expression and normalized to GAPDH to compare the amount of GPR3 at the surface vs. total GPR3 expression. (*) indicates a significant increase in cell surface GPR3 compared to ‘‘GPR3+Dyn WT’’. Significance was determined by Student’s t test (p,0.05). Results are presented as mean 6 S.E.M from 3 separate experiments. doi:10.1371/journal.pone.0065365.g002
  • Figure 3. Inhibition of endocytosis increases intracellular cAMP. A) HEK293 cells were co-transfected with GPR3-HA and pcDNA or with Dyn WT or Dyn K44A. Twenty-four hr after transfection, cells were harvested for cAMP EIA. Bars with different letters are significantly different. Significance was determined by One-way ANOVA followed by Newman-Keuls multiple comparison test (p,0.01).Results are presented as mean 6 S.E.M from 4 separate experiments. B–C) HEK293 cells were co-transfected with GPR3-RFP and CFP-Epac1(dDEP-CD)-YFP and pcDNA, or Dyn WT or Dyn K44A. The YFP/CFP ratios were measured before and after isoproterenol and IBMX treatment. B) Percent change in the YFP/CFP ratio. C) FRET measurements were converted to cAMP levels (mM) as described in the experimental protocol. Bars with different letters are significantly different. Significance was determined by One-way ANOVA followed by Newman-Keuls Multiple Comparison Test (p,0.01). Results were obtained from 15 different GPR3-RFP expressing cells per group. doi:10.1371/journal.pone.0065365.g003
  • Figure 4. Overexpression of GRK2 and b-arrestin-2 decreases cell surface GPR3 expression. A) HEK293 cells were co-transfected with GPR3-HA and pcDNA (2) or GPR3-HA and GRK2 and b-arrestin-2 (+). Twenty-four hr after transfection, cell surface proteins were biotinylated, precipitated, and cell surface expression of GPR3-HA was detected by Western blotting. 0.5 mg of total lysate was used to detect total GPR3 and GAPDH expression. Blot is representative of 3 separate experiments. B–C) Bands corresponding to surface GPR3 and total GPR3 expression were analyzed using densitometry. Densitometric values for total GPR3 expression were normalized to GAPDH. Densitometric values for surface GPR3 was divided by densitometric values for total GPR3 and normalized to GAPDH to compare the amount of GPR3 at the surface vs. total GPR3 expression. (*) indicates a significant decrease in surface/total GPR3 expression as a result of GRK2 and b-arrestin-2 overexpression. Significance was determined by Student’s t test (p,0.05). Results are presented as mean 6 S.E.M. from 3 separate experiments. doi:10.1371/journal.pone.0065365.g004
  • Figure 5. Overexpression of GRK2 and b-arrestin-2 decreases intracellular cAMP levels. A) HEK293 cells were co-transfected with GPR3-HA and pcDNA or GPR3-HA and GRK2 and b-arrestin-2. Twentyfour hr after transfection, cells were harvested for cAMP EIA. Bars with different letters are significantly different. Significance was measured by One-way ANOVA followed by Newman-Keuls Multiple Comparison Test (p,0.05). Results are presented as mean 6 S.E.M from 3 separate experiments. B–C) HEK293 cells were co-transfected with GPR3-RFP, CFP-Epac1(dDEP-CD)-YFP, and pcDNA or GPR3-RFP, CFP-Epac1(dDEPCD)-YFP, GRK2, and b-arrestin-2. The YFP/CFP ratios were measured before and after forskolin and IBMX treatment. B) Percent change in the YFP/CFP ratio. C) FRET measurements were converted to cAMP levels
  • Figure 6. Mutation of S and T residues in the third intracellular loop increases intracellular cAMP. A) Schematic identifying potential serine and threonine residues in the third intracellular loop and C-terminus that could be targeted for regulation by phosphorylation. These residues were mutated to alanine to create 3 mutants: ST/A, S1-6A, and ST/A+S1-6A. B) GPR3-HA WT and mutants were transfected into HEK293 cells and harvested 24 hr later for cAMP EIA. (*) indicates a significant increase in cAMP level compared to ‘‘WT’’. Significance was determined by Repeated Measures ANOVA followed by Dunnett’s Multiple Comparison Test (p,0.01). Results are presented as mean 6 S.E.M. from 6 separate experiments. C) 24 hr after transfection, cell surface proteins were biotinylated, precipitated, and surface expression of GPR3-HA was detected by Western blotting. 0.5 mg of total lysate was used to detect total GPR3 and b-actin expression. Blot is representative of 3 separate experiments: WT, lane 1; ST/A, lane 2; S1-6A, lane 3; ST/A+S1-6A, lane 4. D–E) Bands corresponding to surface GPR3 and total GPR3 expression were analyzed using densitometry. Densitometric values for total expression of GPR3 WT and mutants were normalized to b-actin (D). The densitometric value for surface GPR3 was divided by the densitometric value for total GPR3 expression and normalized to b-actin to compare the amount of GPR3 at the surface vs. total GPR3 (E). (*) indicates a significant decrease in surface expression of GPR3 mutants compared to ‘‘WT’’. Significance was determined by One-way ANOVA followed by Newman-Keuls Multiple Comparison Test (p,0.05). Results are presented as mean 6 S.E.M from 3 separate experiments. doi:10.1371/journal.pone.0065365.g006
  • Figure 7. The effects of GRK2, GRK2-K220R and b-arrestin 2 on GPR3 WT and ST/A activity and surface localization. GPR3-HA WT (A) and ST/A (B) were co-transfected with pcDNA, or GRK2, or GRK2 and b-arrestin-2, or GRK2-K220R, or GRK2-K220R and b-arr-2. Twenty-four hr after transfection, cells were harvested for cAMP EIA. (*) indicates a significant difference in cAMP compared to ‘‘pcDNA’’. Significance was determined by One-way ANOVA followed by Newman-Keuls Comparison Test (p,0.05). Results are presented as mean 6 S.E.M from 3–5 separate experiments. (C) HEK293 cells were co-transfected with GPR3ST/A and pcDNA (2) or GRK2 and b-arrestin-2 (+). Twenty-four hr after transfection, cell surface proteins were biotinylated, precipitated from cell lysates, and analyzed by Western blotting. 0.5 mg of total lysate was used to detect total GPR3 and b-actin expression. Blot is representative of 3 separate experiments. D) Densitometric values for surface GPR3 was divided by densitometric value for total GPR3 and normalized to b-actin to compare the amount of GPR3 at the surface compared vs. total GPR3 expression. (*) indicates a significant decrease in surface/total GPR3 as a result of GRK2 and b-arrestin-2 expression. Significance was determined by Two-way ANOVA followed by Bonferroni Multiple Comparison Test (p.0.05). Results are presented as mean 6 S.E.M from 3 separate experiments. doi:10.1371/journal.pone.0065365.g007

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Lowther, K. M., Uliasz, T. F., Götz, K. R., Nikolaev, V. O., & Mehlmann, L. M. (2013). Regulation of Constitutive GPR3 Signaling and Surface Localization by GRK2 and β-arrestin-2 Overexpression in HEK293 Cells. PLoS ONE, 8(6). https://doi.org/10.1371/journal.pone.0065365

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