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© The Rockefeller University Press,
0021-9525/2001//1381 $5.00
The Journal of Cell Biology, Volume 153, Number 7,
, 2001 1381-1390
Original Article |
Role of the F-Box Protein Skp2 in Adhesion-Dependent Cell Cycle Progression
paganm02{at}med.nyu.edu
Cell adhesion to the extracellular matrix (ECM) is a requirement for proliferation that is typically lost in malignant cells. In the absence of adhesion, nontransformed cells arrest in G1 with increased levels of the cyclin-dependent kinase inhibitor p27. We have reported previously that the degradation of p27 requires its phosphorylation on Thr-187 and is mediated by Skp2, an F-box protein that associates with Skp1, Cul1, and Roc1/Rbx1 to form the SCFSkp2 ubiquitin ligase complex. Here, we show that the accumulation of Skp2 protein is dependent on both cell adhesion and growth factors but that the induction of Skp2 mRNA is exclusively dependent on cell adhesion to the ECM. Conversely, the expression of the other three subunits of the SCFSkp2 complex is independent of cell anchorage. Phosphorylation of p27 on Thr-187 is also not affected significantly by the loss of cell adhesion, demonstrating that increased p27 stability is not dependent on p27 dephosphorylation. Significantly, ectopic expression of Skp2 in nonadherent G1 cells resulted in p27 downregulation, entry into S phase, and cell division. The ability to induce adhesion-independent cell cycle progression was potentiated by coexpressing Skp2 with cyclin D1 but not with cyclin E, indicating that Skp2 and cyclin D1 cooperate to rescue proliferation in suspension cells. Our study shows that Skp2 is a key target of ECM signaling that controls cell proliferation.
Key Words: F-box protein • SCF • Skp2 • p27 • cell adhesion control
© 2001 The Rockefeller University Press
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38 in humans (Cenciarelli et al. 1999; Winston et al. 1999). Fbps contain an F-box, an 
40–amino acid motif that is necessary for the interaction of Fbps with Skp1 (for review see Kipreos and Pagano 2000). Fbps also contain additional protein–protein interaction domains such as leucine-rich repeats and WD-40 domains that are involved in the recognition of phosphorylated substrates. Thus, the substrate specificity of SCFs is dictated by distinct Fbps that target proteins for ubiquitin-mediated degradation. The cyclin-dependent kinase (Cdk) inhibitor p27 negatively regulates cyclin E–Cdk2 and cyclin A–Cdk2 complexes, two kinases necessary for DNA replication. We have reported previously that upon mitogenic stimulation p27 is degraded through the ubiquitin-proteasome pathway (Pagano et al. 1995) and that the ubiquitinylation of p27 is dependent on its Cdk2-mediated phosphorylation and is stimulated by its association to cyclin E–Cdk2 or cyclin A–Cdk2 complexes (Montagnoli et al. 1999). Accordingly, in vivo and in vitro degradation of p27 requires its phosphorylation on Thr-187 by Cdk2 (Sheaff et al. 1997; Vlach et al. 1997; Nguyen et al. 1999). Skp2 is an Fbp first identified together with Skp1 as interactors of the cyclin A–Cdk2 complex, hence the name S phase kinase-associated proteins (Skps). Stimulation of quiescent cells with growth factors induces the expression of Skp2 in late G1 (Carrano et al. 1999; Marti et al. 1999). This induction occurs through a stabilization of Skp2 protein but without activating SKP2 gene transcription (Wirbelauer et al. 2000). We and others have demonstrated that Skp2 is necessary for the ubiquitinylation and subsequent degradation of p27 both in vivo (Carrano et al. 1999; Sutterluty et al. 1999) and in vitro (Carrano et al. 1999; Tsvetkov et al. 1999). In agreement with these findings, interference of Skp2 function by microinjection of an anti-Skp2 antibody into living adherent cells resulted in an inhibition of the entry into S phase (Zhang et al. 1995). Skp2-deficient mice are smaller than littermate controls, and Skp2–/– cells exhibit high levels of p27 and free cyclin E (not bound to Cdk2), polyploidy, and multiple centrosomes (Nakayama et al. 2000). In addition to studies demonstrating that Skp2 is a major player in the degradation of p27 bound to Cdk complexes, there is also evidence of a p27 translational control (Hengst and Reed 1996) and a regulation of p27 subcellular localization (Tomoda et al. 1999).
Cell adhesion to the extracellular matrix (ECM) is required for cell cycle progression through the G1 phase. The cooperative action of cell adhesion and growth factors results in the upregulation of cyclins and the downregulation of Cdk inhibitors, permitting cells to pass through the G1 restriction point and complete the cell cycle (for reviews see Assoian 1997; Giancotti and Ruoslahti 1999). It has been reported that the loss of substratum attachment in fibroblasts induces a stabilization of p27 and an increased association of p27 to Cdk2 with a subsequent decrease in its kinase activity (Fang et al. 1996; Schulze et al. 1996; Zhu et al. 1996; Kawada et al. 1997; Resnitzky 1997). Ultimately, the inhibition of Cdk2 activity results in a G1 arrest. Similar findings were reported for epithelial, arterial smooth muscle, and endothelial cells that were prevented to bind the ECM (Croix et al. 1996; Koyama et al. 1996; Huang et al. 1998). Thus, p27 accumulation plays an important role in inducing a G1 block in response to loss of adhesion. Yet, the mechanism through which p27 accumulates in nonadherent cells is not understood.
The relationship between cell adhesion and cell cycle, particularly the regulation of p27 abundance by ECM–dependent signals, prompted us to test the hypothesis that Skp2 plays a role in this process. The results of these studies are herein presented.
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40 total PDLs. Cells were counted at each passage, and the increase in PDL was calculated as the log2-fold increase in cell number. Rat-6 cells are a clonal line of rat embryo fibroblasts (Krauss et al. 1992). These cells are adhesion-dependent nontumorigenic in nude mice and compared with the widely used Rat-1 cells produce fewer colonies in soft agar and when transfected with activated Ras. Rat-6 cells were cultured in DME plus 5% calf serum. After culturing for 2–3 d in the presence of 0.2% serum, 90% of the cells showed a 2n DNA content by flow cytometry, and 10% of the Rat-6 cell population incorporated BrdU during a 24-h incubation period. This 10% background was subtracted in all analyses of BrdU incorporation to highlight the differences observed under different adhesion conditions (see below). Umbilical vein endothelial cells were obtained from Clonetics Corp. and cultured as described (Tam et al. 1994) for four passages or less (passaged at a 1:4 ratio). Hs913T, 293T, HeLa, and U2-OS cells were obtained from American Type Culture Collection. Rat-6, IMR-90, and endothelial cells were synchronized in G0/G1 by serum starvation for 48 h. To test the effects of lack of adhesion to the ECM, quiescent cells were trypsinized and reseeded on tissue culture–coated Petri dishes (adherent) or Petri dishes coated with 1% agarose (suspension) using 0.5–1 x 106 cells per 10-cm dish. To study the relative effects of fibronectin and growth factors, trypsinized quiescent cells were replated in the presence of a cocktail of purified growth factors (10 ng/ml EGF, 10 ng/ml PDGF, and 10 mg/µl insulin) on tissue culture–coated dishes coated with fibronectin or poly-L-lysine as described (Zhu et al. 1999). Colony formation in soft agar was done as described (Guadagno et al. 1993). For cell cycle analyses, adherent cells were grown on glass coverslips, labeled for 3 h with 10 µm BrdU, rinsed with PBS, and fixed for 10 min in –20°C methanol–acetone (1:1). Fixed cells were rehydrated in PBS at room temperature and processed for cell staining. Suspended cells were also labeled for 3 h with 10 µm BrdU, but during the last 30 min of incubation cells were collected and pulled through a syringe to break up cell clumps. Cells were then plated on glass coverslips that had been coated (4 h at room temperature) with poly-L-lysine (5 µg/ml in PBS; Sigma-Aldrich) for the remaining 20 min and finally fixed as described above. Cells were stained for BrdU as described previously (Ohtsubo et al. 1995) and counterstained with Hoechst to identify all nuclei. The percentage of BrdU-labeled cells (BrdU-positive cells/Hoechst-positive cells x 100) was quantified using a fluorescence microscope. At least 300 cells were counted for each sample, and each experiment was performed at least four times.
Retroviral-mediated Gene Transfer
Packaging GP-293 cells (CLONTECH Laboratories, Inc.) were transfected with retroviral plasmids according to the manufacturer's instructions. 48 h after transfection, the virus-containing medium was collected and supplemented with 8 µg/ml polybrene (Sigma-Aldrich). Then, the culture medium of the target cells was replaced with this viral supernatant for 24 h. This infection process was repeated a second time after a 12-h recovery in normal medium. The percentage of infected cells was quantified by flow cytometry or immunofluorescence. In all cases, >85% of the cells were infected. Multiple genes were introduced sequentially.
Cycloheximide Treatment and Pulse–Chase Analysis
To measure protein half-lives, cells were incubated in the presence of 100 µg/ml cycloheximide (Chx) (Sigma-Aldrich) diluted in DME. Pulse–chase analysis was performed as described (Pagano et al. 1995) with the only difference being that after a 30-min starvation cells were labeled for 30 min with 200 µCi/ml of [35S]methionine and [35S]cysteine (51006; ICN Biomedicals) and chased with medium for the indicated times.
Immunoreagents, Extract Preparation, Immunoblot Analysis, and Kinase Assay
Mouse monoclonal antibodies (Mabs) to Skp2 were produced using bacterial Skp2 produced and purified as described (Schulman et al. 2000). Mabs to Skp2 (Latres et al. 2001), cyclin D1 (Lukas et al. 1994), Ubc3 (Latres et al. 1999), cyclin E (Faha et al. 1993), and rabbit polyclonal antibodies to Skp2 (Carrano et al. 1999), Cul1 (Latres et al. 1999), cyclin A (Pagano et al. 1992), cyclin B (Pagano et al. 1992), cyclin D1 (Lukas et al. 1994), Roc1 (Ohta et al. 1999), and Thr-187 phospho-site p27-specific antibody (Carrano et al. 1999; Montagnoli et al. 1999) were described previously. Mabs to p21 (C24420), p27 (K25020), and Skp1 (P46020) were from Transduction Labs. Mab to Rb (14001A) was from Pharmingen, and Mab to E2F-1 was from Santa Cruz Biotechnology, Inc. (sc-251). Rabbit antibody to cyclin E (sc-481) was from Santa Cruz Biotechnology, Inc. Protein extraction and immunoblot analysis were performed as described (Carrano et al. 1999). Histone H1 kinase reactions were performed as described (Pagano et al. 1992).
Northern Blot Analysis
Total RNA was extracted using Trizol reagent (GIBCO BRL) according to the manufacturer's instructions. For Northern blots, 15 µg of total RNA was loaded per lane and fractionated in a 1% agarose/formaldehyde gel. After transfer onto Hybond N+ membrane (Amersham Pharmacia Biotech), blots were fixed by UV cross-linking and hybridized with a 32P probe specific for human Skp2. A probe specific for glyceraldehyde 3-phosphate dehydrogenase (GAPDH) was used to confirm equal loading. To measure mRNA half-lives, cells were incubated in the presence of 1 µg/ml actinomycin D (Act D) diluted in DME.
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The yeast phosphatase Cdc14 is able to dephosphorylate the Cdk inhibitor Sic1 causing its accumulation because dephosphorylated Sic1 cannot be recognized by the SCF ubiquitin ligase (for review see Zachariae and Nasmyth 1999). Although a human Cdc14 homologue exists (Li et al. 1997), no phosphatase appears to play a role in the stabilization of p27 observed in proliferating cells transferred to suspension. In fact, phosphorylation of p27 on Thr-187 is still detectable in nonadherent cells (Fig. 4). Likely, p27 is still phosphorylated by Cdk2 during the first 4–8 h after replating the cells in suspension, since Cdk2 activity was totally inhibited only between 12 and 16 h as indicated by the state of Rb phosphorylation (Fig. 4, lanes 18–22) and by measuring Cdk2 activity in vitro (data not shown). Despite the fact that p27 is present in its phosphorylated form, p27 accumulates, since it cannot be degraded due to the absence of Skp2. Thus, during cell cycle withdrawal in response to loss of cell adhesion p27 stabilization is not dependent on its dephosphorylation. Interesting, a recent paper shows that p27 accumulates in its phosphorylated form in response to ectopic PTEN expression in PTEN-deficient cells (Mamillapalli et al. 2001). In agreement with our data, these results indicate that p27 accumulation can be regulated by mechanisms other than dephosphorylation.
It has been shown that infecting cells with a recombinant adenovirus expressing Skp2 in serum starved fibroblasts (Sutterluty et al. 1999) or arrested hepatocytes (Nelsen et al. 2001) induces degradation of p27, Cdk activation, and S phase entry. This is in apparent contrast with our results in both fibroblasts (Fig. 2) and thymocytes (Latres et al. 2001) where the presence of Skp2 alone is unable to produce such effects in resting cells. This discrepancy is probably due to the difference in overexpression levels obtained using different viral systems.
Adhesion independence, one of the fundamental properties of cancer cells, is associated with invasiveness and metastasis (Folkman and Moscona 1978). Changes in the expression of cyclins and Cdk inhibitors have been implicated in the adhesion-independent growth of tumor cells (Fang et al. 1996; Orend et al. 1998). Destabilization of p27 that we and others have documented in human epithelial cancers and lymphomas correlates with tumor aggressiveness, poor prognosis (Esposito et al. 1997; Loda et al. 1997; Steeg and Abrams 1997; Piva et al. 1999; Chiarle et al. 2000), and with the presence of metastases (Thomas et al. 1998). We and others have shown recently that Skp2 levels inversely correlate with p27 expression in human lymphomas (Latres et al. 2001), oral squamous cell carcinomas (Gstaiger et al. 2001), colorectal cancers (Hershko et al. 2001), and prostate carcinomas (our unpublished results). Significantly, Skp2 cooperates with activated N-Ras in an in vivo model of lymphomagenesis (Latres et al. 2001). In contrast to all nontransformed cells tested (human, mouse, and rat fibroblasts and human endothelial cells), transformed cells (such as HeLa, 293T, Hs913T, and U2-OS cells) express the same levels of Skp2 regardless of their adhesion conditions (our unpublished results). The data presented herein support and extend previous studies demonstrating that Skp2 is necessary for entering S phase (Zhang et al. 1995; Sutterluty et al. 1999). Furthermore, our findings show that Skp2 is a target of cell adhesion-dependent signaling and together with the high Skp2 levels observed in human cancers suggests a role for Skp2 in the adhesion-independent ability of tumor cells to grow.
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This work was supported by an Irma T. Hirschl scholarship, a Human Frontier Science Program Organization grant (RG0229), National Institutes of Health grants (R01-CA76584 and R01-GM57587), and the Kaplan Comprehensive Cancer Center National Institutes of Health grants (P30-CA16087 and R21-CA66229).
Submitted: 2 March 2001
Accepted: 17 May 2001
Abbreviations used in this paper: Act D, actinomycin D; Adh, adherent; Cdk, cyclin-dependent kinase; Chx, cycloheximide; ECM, extracellular matrix; Fbp, F-box protein; Mab, mouse monoclonal antibody; PDL, population doubling; SCF, Skp1, Cul1, and Fbp complex; Skp, S phase kinase-associated protein; Susp, suspension.
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