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W2000750007 abstract "Article28 September 2006free access Mdm2 is involved in the ubiquitination and degradation of G-protein-coupled receptor kinase 2 Alicia Salcedo Alicia Salcedo Search for more papers by this author Federico Mayor Jr Corresponding Author Federico Mayor Jr Departamento de Biología Molecular and Centro de Biología Molecular ‘Severo Ochoa’, Consejo Superior de Investigaciones Científicas-Universidad Autónoma de Madrid, Madrid, Spain Search for more papers by this author Petronila Penela Corresponding Author Petronila Penela Departamento de Biología Molecular and Centro de Biología Molecular ‘Severo Ochoa’, Consejo Superior de Investigaciones Científicas-Universidad Autónoma de Madrid, Madrid, Spain Search for more papers by this author Alicia Salcedo Alicia Salcedo Search for more papers by this author Federico Mayor Jr Corresponding Author Federico Mayor Jr Departamento de Biología Molecular and Centro de Biología Molecular ‘Severo Ochoa’, Consejo Superior de Investigaciones Científicas-Universidad Autónoma de Madrid, Madrid, Spain Search for more papers by this author Petronila Penela Corresponding Author Petronila Penela Departamento de Biología Molecular and Centro de Biología Molecular ‘Severo Ochoa’, Consejo Superior de Investigaciones Científicas-Universidad Autónoma de Madrid, Madrid, Spain Search for more papers by this author Author Information Alicia Salcedo, Federico Mayor 1 and Petronila Penela 1 1Departamento de Biología Molecular and Centro de Biología Molecular ‘Severo Ochoa’, Consejo Superior de Investigaciones Científicas-Universidad Autónoma de Madrid, Madrid, Spain *Corresponding authors: Departamento de Biología Molecular and Centro de Biología Molecular ‘Severo Ochoa’, Consejo Superior de Investigaciones Científicas- Universidad Autónoma de Madrid, 28049 Madrid, Spain. Tel.: +34 91 497 4865; Fax: +34 91 497 4799; E-mail: [email protected] or E-mail: [email protected] The EMBO Journal (2006)25:4752-4762https://doi.org/10.1038/sj.emboj.7601351 PDFDownload PDF of article text and main figures. ToolsAdd to favoritesDownload CitationsTrack CitationsPermissions Figures & Info G-protein-coupled receptor kinase 2 (GRK2) is a central regulator of G-protein-coupled receptor signaling. We report that Mdm2, an E3-ubiquitin ligase involved in the control of cell growth and apoptosis, plays a key role in GRK2 degradation. Mdm2 and GRK2 association is enhanced by β2-adrenergic receptor stimulation and β-arrestin. Increased Mdm2 expression accelerates GRK2 proteolysis and promotes kinase ubiquitination at defined residues, whereas GRK2 turnover is markedly impaired in Mdm2-deficient cells. Moreover, we find that activation of the PI3K/Akt pathway by insulin-like growth factor-1 alters Mdm2-mediated GRK2 degradation, leading to enhanced GRK2 stability and increased kinase levels. These data put forward a novel mechanism for controlling GRK2 expression in physiological and pathological conditions. Introduction G-protein-coupled receptor kinases (GRKs) and β-arrestins are critical regulators of a wide variety of biological processes. First, these proteins play a major role in the attenuation of signaling mediated by the large family of G-protein-coupled receptors (GPCRs) (Gainetdinov et al, 2004). Besides promoting activation of heterotrimeric G proteins, agonist stimulation of GPCRs leads to receptor phosphorylation by GRKs (Kohout and Lefkowitz, 2003; Penela et al, 2003). This phosphorylation event facilitates binding of β-arrestins to the receptor, resulting in uncoupling from G proteins. Acting as adaptor proteins for components of the endocytic machinery, arrestins also trigger receptor internalization. Therefore, GRKs and arrestins are involved in GPCR desensitization, endocytosis and resensitization (Ferguson, 2001). β-Arrestins and GRKs also regulate other membrane receptor families. It has been reported that β-arrestin binds to ligand-stimulated insulin-like growth factor-1 receptor (IGF1-R), thereby promoting receptor internalization and enhancing IGF-dependent mitogenic signaling (Lin et al, 1998). GRK2, a ubiquitously expressed member of the GRK family, also phosphorylates PDGF-Rβ and reduces receptor activity without altering its downregulation (Freedman et al, 2002; Hildreth et al, 2004). In addition, β-arrestins can act as scaffold molecules that bring different signaling molecules into the receptor complex (reviewed by Lefkowitz and Shenoy, 2005). Likewise, GRK2 has been shown to phosphorylate non-receptor substrates and also to interact with a variety of signaling proteins such as PI3Kγ, Gαq or GIT (Penela et al, 2003, 2006, and references therein). GRK2 also inhibits TGF-β-mediated cell growth arrest and apoptosis by inducing Smad phosphorylation (Ho et al, 2005). Overall, these data suggest that GRK2 may have ‘effector’ functions beyond receptor desensitization. Such functional complexity predicts that alterations in GRK2 levels and/or activity may have important effects on cell signaling. Interestingly, several pathological conditions such as congestive heart failure, hypertension and rheumatoid arthritis (RA), among others, display altered GRK2 expression and function (reviewed by Penela et al, 2003, 2006; Metaye et al, 2005). Whereas different regulatory mechanisms of GRK2 activity and subcellular localization have been described (reviewed by Kohout and Lefkowitz, 2003; Penela et al, 2003), the mechanisms that govern GRK2 cellular levels have only recently began to be addressed. We first described that GRK2 is rapidly degraded by the proteasome pathway, and that β2-adrenergic receptor (β2AR) activation enhances GRK2 ubiquitination and turnover (Penela et al, 1998). We have also shown that agonist-dependent binding of β-arrestin to GPCRs supports GRK2 degradation by allowing the recruitment of c-Src and the phosphorylation of GRK2 on critical tyrosine residues (Penela et al, 2001). MAPK-mediated GRK2 phosphorylation also triggers GRK2 degradation in a process that is again dependent on β-arrestin function (Elorza et al, 2003). Proteasome degradation requires the orchestrated activities of the ubiquitin-activating enzyme (E1), ubiquitin-conjugating enzymes (E2) and ubiquitin ligases (E3) (Pickart, 2001). The specificity of target protein selection is determined by ubiquitin ligases, which interact with their substrates either directly or by means of adaptor molecules. Interestingly, β-arrestins are able to interact with Mdm2, a RING domain-containing E3-ubiquitin ligase involved in the control of tumor suppressor p53 activity (Weissman, 2001). β-Arrestin-mediated recruitment of Mdm2 to several GPCR complexes leads to different β-arrestin ubiquitination patterns, which controls the characteristics of MAPK activation and receptor internalization (Shenoy et al, 2001; Shenoy and Lefkowitz, 2003, 2005; Wang et al, 2003). In this report, we identify Mdm2 as an E3-ubiquitin ligase for GRK2 that is critically involved in kinase ubiquitination and degradation. Moreover, we put forward a new Mdm2-mediated pathway for the modulation of GRK2 cellular levels by IGF-1. Control of GRK2 protein levels by Mdm2 may represent a versatile mechanism for fine-tuning of the expression of this key regulatory kinase by different extracellular signals. Results Mdm2 associates with GRK2 and this process is facilitated by β2AR stimulation and β-arrestin GRK2 is rapidly degraded by the proteasome pathway in response to β2AR agonist stimulation, whereas the turnover of the GRK2-K220R mutant, which lacks kinase activity, is severely impaired (Penela et al, 1998). We have also reported that GRK2 turnover is dependent on β-arrestin function, and that overexpression of either β-arrestin1 or β-arrestin2 is able to promote GRK2-K220R proteolysis (Penela et al, 2001), thus suggesting that these adaptor molecules may recruit some of the factors needed for GRK2 ubiquitination and proteasome degradation. Interestingly, β-arrestins interact with Mdm2, bringing this protein to the plasma membrane β2AR complex, where Mdm2 triggers ubiquitination of β-arrestins and also auto-ubiquitination (Shenoy et al, 2001; Wang et al, 2003). As GRK2 is also part of activated GPCR complexes, we explored the possibility that Mdm2 could act as a GRK2 ubiquitin ligase. Consistent with this idea, we find that endogenous GRK2 and Mdm2 can associate in MCF7 cells, as shown by co-immunoprecipitation experiments using either anti-GRK2 or anti-Mdm2 antibodies (Supplementary data and Supplementary Figure S1A). This suggests that both proteins can be found in the same molecular complex at steady-sate conditions ‘in situ’. We have previously shown that agonist stimulation of β2AR decreases GRK2 half-life from 60 min (basal conditions) to ∼30 min (stimulated turnover) (Penela et al, 1998). Therefore, we tested whether Mdm2 association to GRK2 would be modified by receptor activation. Figure 1A and B shows that β2AR stimulation promotes a rapid and transient increase in endogenous GRK2/Mdm2 association in HeLa cells and in HEK-293 cells coexpressing these proteins. It is worth noting that β2AR stimulation also triggers a rapid and transient association of β-arrestins with Mdm2 (Wang et al, 2003). Interestingly, we find that overexpression of β-arrestin1 increases both the extent and kinetics (maximal co-immunoprecipitation detected at 1–2 min) of GRK2/Mdm2 association upon β-agonist challenge (Figure 1B). A similar effect was observed upon expression of β-arrestin2 (data not shown). Consistent with a key mediator role for arrestins in GRK2 turnover, we find that protein decay of endogenous GRK2 (as assessed by chase experiments in the presence of cycloheximide) was severely delayed in mouse embryonic fibroblasts (MEFs) lacking both β-arrestin1 and β-arrestin2 compared to wild-type MEFs (Figure 1C), indicating that expression of β-arrestins is necessary for normal GRK2 degradation in physiological conditions. Figure 1.(A) Association of endogenous Mdm2 and GRK2. HeLa cells growing in 150 mm dishes were serum-starved for 2 h and incubated with an inverse β-agonist (betaxolol, 10 μM) for 15 min to lessen basal Mdm2/GRK2 association before challenging with 10 μM isoproterenol for the indicated times. Cells were lysed in buffer A as detailed in Materials and methods and lysates subjected to immunoprecipitation with anti-Mdm2 (SMP14) antibody. Immunoprecipitates were resolved by SDS–PAGE and GRK2 associated to the Mdm2 immunocomplex was detected by Western blot analysis with a specific antibody. 1% of the total lysate used for immunoprecipitation was loaded as input signal. (B) The Mdm2/GRK2 association is enhanced by β2AR stimulation and β-arrestin expression. HEK-293 cells were transiently transfected with plasmids encoding GRK2, β2AR, Mdm2 and β-arrestin1 when indicated. Cells were challenged with 10 μM isoproterenol for different times and GRK2/Mdm2 co-immunoprecipitation assessed as detailed in Materials and methods. GRK2 presence in the non-stimulated Mdm2 immunocomplex was taken as the control condition. Data were normalized by total Mdm2 and depicted as mean±s.e.m. of four independent experiments. A representative gel is shown in the bottom panel. (C) Normal decay of GRK2 protein is impaired upon of β-arrestin1 and β-arrestin2 knockdown. GRK2 protein levels were examined by immunoblot analysis in both wild-type and β-arrestin1/2-deficient MEFs upon treatment with cycloheximide (CHX) for the indicated times. The amount of GRK2 at 0 h was defined as 100%, and data normalized by actin protein levels. In both panels, data are the mean±s.e.m. of four independent experiments (*P<0.05). Representative gels are shown. Download figure Download PowerPoint Taken together, these results indicate that Mdm2 can interact with GRK2 in an agonist-dependent manner and suggest that β-arrestin could be a pivotal adaptor to position Mdm2 and/or other ligases in the vicinity of GRK2. Mdm2 promotes GRK2 degradation We next investigated whether Mdm2 could increase the turnover rate of GRK2. First, the stability of GRK2 was determined by pulse–chase assays in HEK-293 cells transiently coexpressing Mdm2 or an empty vector. As shown in Figure 2A, the levels of GRK2 protein decline more rapidly in the presence of Mdm2 (37±1% of [35S]GRK2 protein remaining at 1 h of chase versus 56±3% in the absence of Mdm2 overexpression). Such Mdm2-induced GRK2 proteolysis is blocked by the proteasome inhibitor MG132 (Supplementary data and Supplementary Figure S1B). We have previously shown that the kinase-dead mutant GRK2-K220R displays a severely impaired degradation, probably as a consequence of reduced β-arrestin recruitment to the receptor complex (Penela et al, 2001). Interestingly, Mdm2 is able to associate with this mutant to an extent similar to the wild-type kinase (Supplementary data and Supplementary Figure S1C) and to rescue its defective turnover (Figure 2A, 60±1% of GRK2-K220R remaining at 1 h of chase compared to 92+5% in the absence of Mdm2 expression). Overall, these data are consistent with a role for Mdm2 in the agonist-induced, β-arrestin-mediated GRK2 degradation. Figure 2.(A) Mdm2 increases degradation of GRK2 and of a slow-turnover GRK2 mutant. HEK-293 cells were transiently transfected with wild-type GRK2 or the GRK2-K220R mutant in the presence or absence of Mdm2, and kinase turnover assessed by pulse–chase experiments as described in Materials and methods. 35S-labeled proteins immunoprecipitated with the anti-GRK2 antibody AbFP2 were resolved by SDS–PAGE followed by fluorography and densitometry. 35S-labeled GRK2 band densities were then normalized to total GRK2 present in the immunoprecipitates, as determined by Western blot analysis. Data are mean±s.e.m. of 3–4 independent experiments performed in duplicate, *P<0.05, **P<0.01. A representative gel autoradiography is shown. (B, C) Effect of LMB treatment on GRK2 turnover. HEK-293 cells transfected with GRK2 and Mdm2 or an empty vector were treated with LMB or vehicle before and during pulse–chase experiments as detailed in Materials and methods, and GRK2 turnover determined as in previous figures. Data are the mean±s.e.m. of three independent experiments performed in duplicate, *P<0.05, **P<0.01. Representative fluorographs are shown. In panel C, endogenous GRK2 expression levels were determined by immunoblot analysis in lysates from MCF7 cells treated for different times with LMB. Data are corrected for actin expression and depicted as percentage of control. *P<0.05, ***P<0.001. A representative blot is shown. Download figure Download PowerPoint We next analyzed the effect of leptomycin B (LMB) on GRK2 stability. LMB, a drug that blocks nuclear export, has been shown to inhibit Mdm2 nuclear–cytoplasmic shuttling, thus leading to an increased nuclear localization of Mdm2 (Lain et al, 1999). As shown in Figure 2B, the turnover of transiently transfected GRK2 in HEK-293 is significantly retarded in the presence of LMB (80±10% of protein remaining at 1 h of chase compared with 57±5% in control conditions). This treatment does not affect GRK2 localization in our experimental conditions (data not shown), thereby ruling out that this effect is caused by altered kinase distribution. Moreover, the enhanced GRK2 turnover observed upon coexpression of Mdm2 (34±2% of labeled kinase remaining) was not observed in the presence of LMB (60±6% of protein remaining), thus suggesting that the effects of LMB on GRK2 stability are due to the impairment of Mdm2 function and/or localization. In line with this notion, LMB promotes a time-dependent increase (in the range of ≈1.4- to 2-fold) of endogenous GRK2 steady-state levels in MCF7 cells (Figure 2C), consistent with a physiological role for Mdm2 in GRK2 degradation. Mdm2 modulates GRK2 ubiquitination We have previously reported that agonist stimulation of β2AR promotes an increase in GRK2 polyubiquitination, consistent with its stimulatory effect on kinase turnover (Penela et al, 1998). As β2AR activation triggers Mdm2/GRK2 association, we next investigated whether Mdm2 would modulate GRK2 ubiquitination. HEK-293 cells were transiently transfected with β2AR, HA-tagged ubiquitin and GRK2 in the presence or absence of Mdm2. Interestingly, both basal and agonist-induced GRK2 polyubiquitination are markedly enhanced upon Mdm2 expression (Figure 3A), supporting a role for Mdm2 as an E3-ubiquitin ligase for GRK2. Figure 3.Mdm2 promotes GRK2 ubiquitination. (A) Wild-type GRK2, HA-ubiquitin and β2AR expression plasmids were transfected together with Mdm2 or an empty vector into HEK-293 cells. After 2 h of serum starving, cells were incubated with or without 10 μM isoproterenol for 15 min and lysed for ubiquitination assays as described in Materials and methods. The different GRK2 species present in the ubiquitin immunoprecipitates are indicated. Asterisk and arrowhead indicate mono- and bi-ubiquitinated GRK2 forms (see text for details). Blots depicting expression levels for Mdm2 and GRK2 in total lysates are shown. (B) Both basal and agonist-stimulated ubiquitination of endogenous GRK2 are blocked in either Mdm2- or β-arrestin-deficient cells. ∼50 × 106 wild-type MEFs or MEFs devoid of Mdm2 or β-arrestin proteins were serum-starved and challenged or not with 10 μM isoproterenol for 15 min. Cells were processed as indicated above and ubiquitinated GRK2 species were analyzed by immunoprecipitation of endogenous GRK2 with a specific monoclonal anti-GRK2 antibody (c5/1.1) and detection of endogenous ubiquitin conjugates with anti-ubiquitin antibody FK2. Membranes were stripped and immunoblotted (right panel) with a specific polyclonal anti-GRK2 antibody (C-15) to confirm equal GRK2 loading in each condition. (C) Mutation of critical lysine residues in the N-terminus of GRK2 impairs kinase ubiquitination in the presence of Mdm2. Wild-type GRK2 or the GRK2- K19,20,30,31R mutant was cotransfected with ubiquitin plasmids in the presence or absence of Mdm2 into HEK-293 cells and the kinase ubiquitination pattern was analyzed as above. Expression levels of GRK2 and Mdm2 were assessed in lysates by Western blot analysis. Gels in all panels are representative of 2–3 independent experiments. Download figure Download PowerPoint The GRK2 ubiquitination patterns induced by receptor stimulation or Mdm2 expression are very similar. The bands of modified kinase migrating at 80 kDa (asterisk) and immediately above (arrowhead) appear to correspond to monoubiquitinated forms of GRK2, whereas the smeared bands in the 97–200 kDa range correspond to polyubiquitinated species of GRK2 (see Supplementary data and Supplementary Figure S2A). To further substantiate the involvement of Mdm2 as a GRK2 ubiquitin ligase, we compared the ubiquitination of endogenous kinase in wild-type MEFs (expressing endogenous Mdm2 levels) or in MEFs from Mdm2-deficient mice. As shown in Figure 3B, in wild-type MEFs, isoproterenol challenge promotes a marked increase in endogenous GRK2 ubiquitinated species. It must be noted that such basal and agonist-promoted GRK2 ubiquitination pattern is similar to that observed in a heterologous system with overexpressed proteins (see Figure 3A). Interestingly, in Mdm2-deficient MEFs, basal GRK2 ubiquitination was attenuated, whereas the agonist-induced component was severely inhibited, indicating a pivotal role for Mdm2 in this process. Moreover, a similar impairment of GRK2 ubiquitination results also from the absence of β-arrestins, consistent with their role as mediators of the ligase recruitment to GRK2 (Figure 3B). To explore the specificity of GRK2 ubiquitination by Mdm2, we sought to identify lysine residues in GRK2 critical for supporting Mdm2-dependent ubiquitin attachment. Multiple lysine-to-arginine changes in lysine-rich regions have been reported to result in resistance to proteasomal degradation in several proteins, including p53, the classical Mdm2 target (Rodriguez et al, 2000). As GRK2 lysine residues at positions 19, 21, 30 and 31 are in close proximity to the initial cleavage site on GRK2 by the proteasome (Penela et al, 1998), we tested the ubiquitination and degradation pattern of a GRK2-K19,21,30,31R mutant transiently coexpressed in HEK-293 cells with the β2AR and a tagged HA-ubiquitin construct. Mutation of these lysine residues leads to a clear reduction in the extent and pattern of ubiquitination as compared to wild-type GRK2, both in basal conditions and upon receptor challenge (Supplementary data and Supplementary Figure S2B). Moreover, in contrast to wild-type kinase, the presence of Mdm2 does not modify the extent of GRK2-K19,21,30,31R ubiquitination (Figure 3C), despite the fact that this mutant can associate with Mdm2, as demonstrated by co-immunoprecipitation experiments (Supplementary data and Supplementary Figure S3A). Overall, these results suggest that at least some of these lysine residues in GRK2 are targeted by Mdm2 in an agonist-dependent manner. Mdm2-mediated ubiquitination of GRK2 lysine residues 19, 21, 30 and 31 is critical for kinase degradation We next investigated the consequences of impairing Mdm2-dependent ubiquitination of GRK2. The GRK2-K19,21,30,31R mutant was transiently coexpressed in HEK-293 cells with the β2AR, and the kinase turnover was analyzed by pulse–chase assays. As shown in Figure 4A, degradation of this mutant was clearly delayed in basal conditions, with a half-life three-fold longer than that of wild-type GRK2, consistent with its reduced ubiquitination. Moreover, receptor stimulation does not significantly enhance GRK2-K19,21,30,31R degradation (data not shown). It should be noted that this mutant displayed similar subcellular distribution and kinase activity as compared to wild-type GRK2 (Supplementary data and Supplementary Figure S3B and C), thus ruling out the possibility that the altered degradation might arise from changes other than impaired ubiquitination. In this regard, the slower turnover of this mutant was also blocked in the presence of proteasome inhibitors (data not shown), thus confirming that mutation of these lysine residues severely retards but does not change the proteolytic pathway responsible for degrading the protein. Figure 4.N-terminal lysine residues are critical for Mdm2-mediated GRK2 degradation. (A) Turnover of wild-type GRK2 and GRK2-K19,20,30,31R mutant proteins was assessed by pulse–chase experiments in HEK-293 cells as described in Materials and methods and Figure 2. (B) Similar experiments were performed in cells cotransfected with an Mdm2 construct. In both panels, data are mean±s.e.m. from three to four independent experiments (**P<0.01), and representative fluorographies are shown. Download figure Download PowerPoint Interestingly, overexpression of Mdm2 is unable to accelerate GRK2-K19,21,30,31R degradation (88±3% of mutant protein remaining in the absence of Mdm2 compared with 86±4% in its presence; Figure 4B). These results indicate that the ubiquitination of defined amino-terminal lysine residues of GRK2 is critical for proper kinase degradation and also strongly suggest that the agonist-dependent increase in GRK2 turnover involves the E3 ligase Mdm2-dependent modification of these residues. GRK2 turnover rate is markedly decreased by Mdm2 knockdown In order to substantiate the regulatory role of Mdm2 in GRK2 stability, we next examined whether degradation of ectopically expressed GRK2 is altered in Mdm2-deficient MEFs. Figure 5A shows that the GRK2 protein decay is severely impaired in the absence of Mdm2, with 98±9% of labeled GRK2 remaining after 1 h of chase, which resembles the altered kinase degradation caused by abrogation of its Mdm2-dependent ubiquitination (Figure 4A and B). Interestingly, restoration of Mdm2 expression in the Mdm2-deficient MEFs rescues GRK2 turnover (Figure 5A), leading to a proteolysis pattern close to that observed for GRK2 in different cellular settings with intact Mdm2 expression (Figure 3; Penela et al, 2001). To further confirm that Mdm2 contributes to degradation of GRK2 in physiological conditions, we compared the protein decay of endogenous kinase by chase experiments in the presence of cycloheximide in both wild-type and Mdm2-deficient MEFs. Figure 5B shows that the degradation rate of GRK2 in MEFs lacking Mdm2 is slower than in wild-type MEFs in these conditions. Moreover, the steady-state expression of endogenous GRK2 is higher in Mdm2-deficient MEFs than in Mdm2-intact cells (compare lane 6 versus lane 1 in the lower panel of Figure 5B). Overall, these results indicate that Mdm2 is involved in degradation of GRK2 in endogenous conditions, and that this ligase plays a critical role in maintaining basal GRK2 turnover. Figure 5.GRK2 turnover is blocked in Mdm2-deficient cells. (A) Mdm2-null MEFs were transfected with wild-type GRK2 in the presence or absence of Mdm2. Degradation of the heterologous GRK2 protein was assessed after 1 h of chase as in previous figures. (B) Stability of endogenous GRK2 is increased in the absence of Mdm2 expression. GRK2 protein levels were examined by immunoblot analysis in both wild-type and Mdm2-deficient MEFs upon treatment with cycloheximide (CHX) for the indicated times. The amount of GRK2 at 0 h was defined as 100%, and data normalized by actin protein levels. In both the panels, data are the mean±s.e.m. of four independent experiments (*P<0.05, **P<0.01). Representative gels are shown. Download figure Download PowerPoint GRK2 stability is modulated by IGF-1 signaling via Mdm2 and the PI3K/Akt pathway The experiments shown above demonstrate that GRK2 degradation requires Mdm2-dependent ubiquitination, and suggest that stimulation of GPCRs such as β2AR may enhance GRK2 turnover by facilitating the interaction of GRK2 with a β-arrestin-recruited pool of Mdm2. It has been recently reported that Mdm2 can also be recruited by β-arrestin molecules in response to activation of tyrosine kinase receptors such as the IGF1-R, thus promoting degradation of several targets including the receptor itself (Girnita et al, 2005). Therefore, we asked whether IGF1-R activation might elicit some modulatory effects on GRK2 stability. To this end, the degradation rate of endogenous GRK2 was determined by pulse–chase assays in the breast human carcinoma cell line MCF7, which expresses endogenous IGF1-R. Under normal conditions, GRK2 is degraded in MCF7 cells with a time course similar to that observed for this kinase in other cell types, and GRK2 half-life remains essentially unaltered when chasing MCF7 cells in low serum medium (data not shown), an experimental condition selected to analyze the potential effects of IGF-1 stimulation. Surprisingly, GRK2 degradation was markedly delayed at all chase points examined in cells challenged with IGF-1 as compared to untreated cells (∼1.3-fold of protein decay between 0.5 and 2 h of chase in the presence of IGF-1 versus ∼2-fold decay in its absence) (Figure 6A). Recently, several groups have reported that Akt interacts with and phosphorylates Mdm2 in response to activation of IGF1-R (Mayo and Donner, 2001; Feng et al, 2004) promoting its nuclear shuffling. Therefore, we hypothesized that Akt phosphorylation of the E3 ligase could impair Mdm2-dependent GRK2 degradation. To test this hypothesis, we performed pulse–chase assays in HEK-293 cells expressing GRK2 with a constitutively active mutant of Akt (Akt-myr). As shown in Figure 6B, GRK2 degradation is clearly diminished in the presence of Akt-myr as compared to the turnover of GRK2 alone (74±8% of 35S-labeled kinase remaining at 1 h of chase versus 49±3%, respectively). Interestingly, the expression of Akt-myr causes a dramatic change in the GRK2 proteolysis promoted by Mdm2 (63±15% of protein remaining after 1 h of chase compared to 26±3% in the presence of Mdm2 only) (Figure 6B). These findings suggest that activation of Akt by IGF-1 signaling can prevent the effect of Mdm2 on GRK2 turnover, thus leading to kinase stabilization. Figure 6.IGF receptor activation and Akt activity promote GRK2 stabilization. (A) Turnover of endogenous GRK2 was analyzed in MCF7 cells as detailed in Materials and methods in the presence of 50 ng/ml of IGF-1 or vehicle. Labeled proteins were immunoprecipitated with a specific anti-GRK2 antibody (C5/1.1). The density of the 35S-labeled GRK2 band after the pulse period was taken as 100%. Data are mean±s.e.m. of 3–5 independent experiments. *P<0.05; **P<0.01. A representative fluorography is shown. (B) HEK-293 cells were transfected with different combinations of GRK2, Mdm2 and a constitutively active Akt mutant (Akt-myr) as indicated. GRK2 degradation rate was determined by pulse–chase analysis. Results (mean±s.e.m.) from three independent experiments are shown. *P<0.05. Download figure Download PowerPoint In line with these data, steady-state expression levels of endogenous GRK2 increase progressively in MCF7 cells upon treatment with IGF-1 as assessed by immunoblot analysis (Figure 7A). The increase was apparent after 4 h of incubation and attained a value of ≈two-fold at 24 h. Interestingly, the peak activation of Akt upon IGF-1 challenge precedes the burst in GRK2 levels (Figure 7A, lower panel). Moreover, Akt-dependent phosphorylation of Mdm2, as detected with specific phospho-antibodies, correlates with the timing of GRK2 accumulation (Figure 7A, lower panel). This suggests that modification of Mdm2 by the PI3K/Akt pathway abrogates ligase activity towards GRK2 and therefore leads to protein accumulation. Consistent with this notion, IGF-1-mediated GRK2 upregulation was impeded in the presence of a PI3K inhibitor (Figure 7A), which also abolishes Akt activation and Mdm2" @default.
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W2000750007 date "2006-09-28" @default.
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W2000750007 title "Mdm2 is involved in the ubiquitination and degradation of G-protein-coupled receptor kinase 2" @default.
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W2000750007 doi "https://doi.org/10.1038/sj.emboj.7601351" @default.
W2000750007 hasPubMedCentralId "https://www.ncbi.nlm.nih.gov/pmc/articles/1618114" @default.
W2000750007 hasPubMedId "https://pubmed.ncbi.nlm.nih.gov/17006543" @default.
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