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p38 Mitogen-Activated Protein Kinase Integrates Signaling Crosstalk between Ras and Estrogen Receptor to Increase Breast Cancer Invasion

Departments of ¹ Radiation Oncology, ² Pharmacology and Experimental Therapeutics, and ³ Pathology and ⁴ Program in Molecular Biology, Loyola University Chicago, Maywood, Illinois and ⁵ Department of Pharmacology and Toxicology, Medical College of Wisconsin, Milwaukee, Wisconsin

Requests for reprints: Guan Chen, Department of Pharmacology and Toxicology, Medical College of Wisconsin, 8701 Watertown Plank Road, Milwaukee, WI 53226. Phone: 414-456-8636; Fax: 414-456-6545; E-mail: gchen{at}mcw.edu.

	Abstract

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Ras is believed to stimulate invasion and growth by different effector pathways, and yet, the existence of such effectors under physiologic conditions has not been shown. Estrogen receptor (ER), on the other hand, is both anti-invasive and proliferative in human breast cancer, with mechanisms for these paradoxical actions remaining largely unknown. Our previous work showed an essential role of p38 mitogen-activated protein kinase in Ras transformation in rat intestinal epithelial cells, and here, we show that p38 integrates invasive antagonism between Ras and ER to increase human breast cancer invasion without affecting their proliferative activity. Ras positively regulates p38 expression, and p38 in turn mediates Ras nonmitogenic signaling to increase invasion. Expression of the Ras/p38 axis, however, is trans-suppressed by ER that inhibits invasion and stimulates growth also by distinct mechanisms. Analysis of ER and its cytoplasmic localized mutant reveals that ER additionally binds to p38 protein, leading to its specific down-regulation in the nuclear compartment. A p38-antagonistic activity of ER was further shown in a panel of breast cancer cell lines and was shown independent of estrogens by both ER depletion and ER expression. These results revealed that both Ras and ER use distinct pathways to regulate breast cancer growth and invasion, and that p38 specifically integrates their antagonistic activity to stimulate cell invasion. Selective targeting of p38-dependent invasion pathways may be a novel strategy to control breast cancer progression. (Cancer Res 2006; 66(15): 7540-7)

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

 
Two defining hallmarks of cancer are uncontrolled proliferation and increased invasion (1). Although increased proliferation is frequently associated with enhanced invasion (2), recent evidence suggests that these two events are distinct (3–6). Ras protein is involved in human malignancies through multiple processes that include increased proliferation, enhanced invasion, and altered cytoskeleton organization (2). Although studies with Ras effector domain mutants suggest a specific role of individual Ras effectors/pathways in these processes (7, 8), the existence of such effectors under physiologic conditions remains unproven. Ras protein is overexpressed in up to 60% of human breast cancer (1, 9), and dissecting Ras mitogenic signaling from its invasive activity is, therefore, critical in understanding its promoting roles in breast cancer progression.

Estrogen receptor (ER) is a nuclear transcription factor that regulates gene expression through binding to specific estrogen-responsive elements (ERE) on a target gene promoter. ER is proliferative in mammary tissues and consequently implicated in the etiology of breast cancer (10, 11). Paradoxically, ER inhibits breast cancer in vitro invasion and in vivo metastasis (12, 13). Furthermore, higher levels of ER protein expression in human breast cancers correlate negatively with clinical metastasis but positively with the prognosis (14, 15). These results together indicate that ER may use distinct pathways to stimulate breast cancer growth and to inhibit its invasion/metastasis.

ER may regulate breast cancer progression through crosstalk with Ras/mitogen-activated protein kinase (MAPK) signaling. Activation of the Ras/extracellular signal-regulated kinase (ERK) pathway downstream of growth factor receptors such as epidermal growth factor receptor (EGFR) increases both cell proliferation and invasion (4, 16). However, forced Ras expression in ER⁺ breast cancer cells inhibits ER activity (17), and expression levels of EGFR and/or Ras proteins are higher in ER^– and/or metastatic breast cancers (18–20). These results suggest that ER and Ras cooperate in stimulating growth but antagonize each other in regulating invasion, and dissecting their crosstalk may contribute to understanding breast cancer progression.

MAPKs consist of ERK, c-Jun NH₂-terminal kinase, and p38 cascades. ERK activity is essential for Ras-induced proliferation/transformation (21, 22), whereas p38 is inhibitory to Ras activity (23–25). In response to Ras-induced invasion, however, both ERK and p38 are required in this process (26). Although these different p38 effects on Ras-induced proliferation and invasion are not understood, some p38 family members may have distinct activity in these regulations. For example, p38 isoform proteins can be either cooperative or antagonistic in regulating gene expression and cell proliferation (27, 28). Studies of p38 isoform-specific effects may contribute to understanding different Ras-p38 signaling interactions in regulating cell proliferation and invasion.

The p38 family consists of four isoforms: , ß, , and (29). p38, also called stress-activated protein kinase 3 or ERK6, shares about 60% identity with p38 and p38ß (30, 31). In contrast to the ubiquitously expressed p38, p38 is only detectable in certain normal tissues (30, 31). Recent studies, however, show that p38 protein is highly expressed in several human malignant cell lines (27, 32, 33), indicating its possible contributing role in cancer development. Indeed, our recent studies showed that Ras activates p38 by increasing its expression in rat intestinal epithelial (IEC-6) cells, and induced p38, albeit nonmitogenic by itself, is required for Ras transformation (34). Specific roles of p38 in Ras-associated human cancers, however, remain to be established. Because Ras plays critical roles in increasing breast cancer progression (2), p38 may function as a Ras effector in this regulation.

Here, we sought to test the hypothesis that the Ras/p38 axis may exist in human breast cancer and thereby regulate breast cancer progression in coordination with ER protein. Our results revealed that in human breast cancer, Ras dictates p38 expression, which in turn mediates Ras nonmitogenic signaling to stimulate cell invasion. The invasive activity of the Ras/p38 axis, however, is antagonized by ER protein through trans-repression, and ER can additionally disrupt p38 protein through direct binding. These results suggest an invasive role of p38 in human breast cancer through integrating Ras proinvasive and ER anti-invasive signaling.

	Materials and Methods

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cDNA constructs. Recombinant adenovirus vector (Ad-Vect) and vector-containing oncogenic H-Ras (Leu⁶¹, L61) or dominant-negative H-Ras (Asn¹⁷, N17) were provided by Dennis Stacey (35). Adenovirus ß-gal (ad-ß-galactosidase), ad-MKK6, and ad-p38 were described elsewhere (32). Retroviral vector pLHCX (provided by Dan Mercola; ref. 36) was used to express p38. To deplete endogenous protein, a retroviral vector pSUPER (pSR; ref. 37) was used (target sequence for sip38 was 5'-AAGGAGATCATGAAGGTGACG-3' and for siER was 5'-AAGAGGAGGGAGAATGTTGAA-3') using a luciferase gene sequence as a control (5'-CGTACGCGGAATACTTCGA-3'; ref. 34). Human ER cDNA and ERE luciferase reporter (ERE-Luc, four ERE repeats upstream of a luciferase gene) were provided by David Shapiro (38). ER site–directed mutagenesis (T311A) was carried out by a PCR-based technique using the QuickChange mutagenesis kit (Stratagene, La Jolla, CA) with primer sequences as previously published (39). All mutations generated were confirmed by DNA digestion with restriction enzymes and DNA sequencing.

Cell culture, reagents, and Tet-inducible ER expression. MEM and other reagents for cell culture were purchased from Life Technologies (Gaithersburg, MD). Protein-Sepharose G beads and Cy3- and FITC-labeled second antibodies were obtained from Zymed (South San Francisco, CA). p38 isoform–specific antibodies were described previously (27, 34), and their specificity was further confirmed by antibodies from BD Clontech (Palo Alto, CA). ERK1/2 and ER antibodies were from Santa Cruz Biotechnology (Santa Cruz, CA), whereas phosphorylated p38 (p-p38) and phosphorylated-ERK (p-ERK) antibodies were from Cell Signaling (Beverly, MA). Mouse pan-Ras antibody was purchased from Oncogene Research Products (San Diego, CA). Human breast cancer cell lines [ER⁺: MCF-7 and 47D; ER^–: MDA-MB-231 (231) and MDA-MB-468 (468)] were obtained from the American Type Culture Collection (ATCC, Manassas, VA) and maintained in MEM containing 10% fetal bovine serum (FBS) and antibiotics at 37°C with 5% CO₂. The Tet-on expression system (T-Rex) was purchased from Invitrogen (San Diego, CA) and used to express human ER or ER/T311A in 231 cells as previously described (40). To evaluate effects of estrogens, cells were cultured with 10% charcoal-treated serum in phenol-free medium for 48 hours and then treated with 10 nmol/L estrogens for additional 24 hours.

Transfection, viral infection, reporter assays, and small interfering RNA experiments. ERE-Luc was transiently transfected by calcium phosphate into Tet-ER cells, which were then incubated with and without Tet for an additional 24 hours before the reporter assay using dual luciferase kit (41). For adenoviral infection, cells were infected with ad-vector or ad-L61/ad-N17 Ras in no serum medium for 4 hours and cultured in normal medium for 24 hours for protein expression and migration assays. In the case of retroviral infection, pSUPER (pSR-Lucif, pSR-sip38, and pSR-siER) and pLHCX (Vector and p38; refs. 24, 34) were transfected into Phoenix-Ampo retrovirus packaging cells (ATCC), and supernatants were used to infect target cells. Typically, cells were analyzed for protein or RNA expression at 24 to 48 hours.

Invasion, cell growth, and data analysis. Invasion assays were carried out using the BioCoat Matrigel Invasion Chamber (BD Biosciences, Bedford, MA) according to the manufacturer's instruction. Briefly, 2.5 x 10⁵ cells in serum-free medium were plated into each chamber, which was placed into the six-well plate containing 20% FBS and incubated for 22 hours, at 37°C, 5% CO₂. Tetracycline (Tet) was added 2 hours later to both inserts and the bottom well to induce ER expression. For infection, cells are replated for invasion assay 24 hours after removal of virus-containing medium. Following incubation, the noninvaded cells on the upper surface of membrane were removed, and the invaded cells on the lower surface were washed, fixed, and stained with crystal violet. The number of invaded cells from 13 to 20 representative fields was counted manually under a phase-contrast microscope, normalized to the respective control. To further verify these results, some crystal-stained attached cells were solubilized with 10% acetic acid and quantitated at 600 nm (42). For cell growth assay, cells were plated with or without Tet and pulsed labeled with [³H]thymidine, and the incorporated radioactivity was determined as previously described (41). All results were analyzed by Student's t test for statistically significant difference.

Immunostaining, immunoprecipitation, glutathione S-transferase pulldown, and cell fractionation/Western and Northern blot assays. For immunostaining, cells were plated on coverslips and fixed in 3.7% formaldehyde. After permeabilized in a buffer containing 0.5% Triton X-100 and 0.5% NP40, cells were blocked in 3% bovine serum albumin in PBS. A mouse monoclonal anti-flag (M2, Sigma, St. Louis, MO) and anti-ER (F10) antibody at 1:100 were used for flag-p38 and ER staining, as previously described (34, 40). For immunoprecipitation, cell lysates were incubated with a goat p38 antibody, and the precipitates were examined for ER protein by Western blot. For glutathione S-transferase (GST) pulldown assay, GST, GST-ER and GST-ER/T311A proteins were expressed in Escherichia coli BL21 and purified using reduced glutathione-agarose beads (23).

To examine protein expression, cells were directly lysed in 1x loading buffer. After heating, samples were separated on SDS-PAGE and transferred to a nitrocellulose membrane for detection of the molecule of interest using enhanced chemiluminescence kit. For cell fractionations, cytoplasmic and nuclear fractions were prepared as previously described (43). For Northern blot, total RNA was prepared by TRIzol (Invitrogen) and separated by agarose gel. p38 and p38 probe was prepared from their corresponding human cDNAs in pcDNA3 vector by enzymatic digestion and/or PCR (34). The probe was labeled with [³²P]dCTP using High Primer kit (Roche Molecular Biochemical, Indianapolis, IN). The Northern blots were standardized for equal RAN loading using the UV fluorescence of the 18S rRNA band from the same membrane.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

 
Ras positively regulates p38 expression independent of ERK and/or p38 phosphorylation, whereas ER trans-suppresses Ras/p38 in human breast cancer. Previous studies have shown that both transient and stable Ras expressions induce p38 protein expression in IEC-6 cells (34). To determine whether Ras regulates p38 expression in human breast cancer, adenovirus-mediated gene delivery was used to express oncogenic H-Ras (L61) and the dominant-negative mutant (N17; ref. 35) in ER^– 231 human breast cancer cells. Following infections, cells were analyzed for protein expression and phosphorylation. Consistent with the positive regulatory effect in IEC-6 cells (34), L61 increases whereas N17 decreases p38 but not p38 protein expression compared with the control ß-gal infection (Fig. 1A and B ). In contrast to the p38 induction in IEC-6 cells, Ras-regulating p38 protein expression does not associate with significant alterations in ERK and/or p38 phosphorylations (Fig. 1A and B), in agreement with a recent observation of Ras activity dissociating with ERK phosphorylation in human breast cancer cells (44). These results reveal a determinant role of Ras activity in p38 protein expression in human breast cancer independent of ERK/p38 phosphorylation and indicate a possible role of p38 in Ras regulating breast cancer progression.

View larger version (22K): [in this window] [in a new window]   Figure 1. Ras positively regulates p38 protein expression independent of ERK phosphorylation, whereas both Ras and p38 protein expression is trans-suppressed by ER in human breast cancer cells. A, Ras inhibition suppresses p38 expression without affecting ERK/p38 phosphorylation. ER– 231 cells were infected with control adenovirus (Ad-ß-gal) or virus expressing dominant-negative Ras (Ad-N17) for 4 hours and incubated for an additional 24 hours before analyzed for protein expression by Western blot. B, Ras activation induces p38 expression without stimulating ERK phosphorylation. Cells were infected with Ad-ß-gal or virus expressing oncogenic H-Ras (Ad-L61) as in (A) and examined for protein expression. C and D, ER inhibits Ras/p38 protein expression dependent of its transcription activity. Cells were cultured with and without Tet for the indicated time to induce wild-type (C) and the mutant ER expression (D), and their effects on Ras/p38 protein expression were examined by Western. Representative from three separate experiments.

p38 transmits Ras nonmitogenic signaling to promote ER^– breast cancer invasion. The Ras determinant role in p38 protein expression prompted us next to explore if p38 acts as a Ras effector to execute its functions in regulating breast cancer invasion and growth. To assess roles of endogenous Ras in these regulations, ER^– 231 cells were infected with Ad-ß-gal or Ad-Ras (N17), and its effects on cell invasion/growth were determined. Functional aspects of endogenous p38 in these processes, on the other hand, were analyzed by small interfering RNA–mediated p38 depletion (34). As expected, inhibition of Ras activity by N17 substantially decreases Matrigel cell invasion and DNA synthesis (P < 0.001 for both cases; Fig. 2A-C ), indicating that Ras activity is required for both processes (26, 46). In contrast to the Ras inhibition, p38 depletion only inhibits invasion (P < 0.01) without affecting thymidine incorporation (P > 0.05, Fig. 2A-C), suggesting a specific role of p38 in stimulating cell invasion. These results indicate that although p38 is downstream of Ras, they have common and distinct roles in regulating breast cancer invasion and growth.

View larger version (27K): [in this window] [in a new window]   Figure 2. Endogenous Ras activity is required for both proliferation and invasion, whereas p38 only transmits nonmitogenic Ras signaling to stimulate invasion. A, adenovirus-mediated N17 expression and small interfering RNA–induced p38 depletion. Cells were infected with either adenovirus (Ad-ß-gal or Ad-N17) or retrovirus (pSR-Lucif, control retrovirus; pSR-sip38, small interfering RNA retrovirus) and incubated for 24 hours before Western analysis. B, both Ras inhibition and p38 depletion inhibit cell invasion. Cells were plated for invasion assay after infection, and invaded cells were counted and normalized to respective controls. Columns, mean of 15 fields (P < 0.01 for N17 and sip38 versus their respective controls); bars, SD. Similar results were obtained from additional two experiments. C, Endogenous Ras but not p38 is required for cell proliferation. Cells were infected as above, and cell proliferation was estimated by thymidine incorporation. Columns, mean of three experiments (P < 0.05 only for Ad-N17 versus Ad-Vect); bars, SD. D, N17 and p38 overexpression. ER– 231 cells were infected either with adenovirus (Vect, N17) and/or pLHCX retrovirus (Vect, p38) and analyzed for protein expression 24 hours later. E, p38 overexpression rescues N17-mediated invasion inhibition. Cells were coinfected with Ad-N17 with and without pLHCX-p38 and assessed for cell invasion as described above. Columns, mean of 13 fields (P < 0.01 for p38 versus Vect, N17 versus Vect, and for N17 versus p38 + N17); bars, SD. Similar results are obtained from one additional experiment. F, high levels of p38 protein expression do not overcome N17-induced growth inhibition. Columns, mean of three separate experiments (P < 0.05 for N17 versus Vect, but P > 0.05 for p38 versus Vect and N17 + p38 versus N17); bars, SD.

ER regulates breast cancer growth and invasion by distinct pathways. The above results showed that Ras stimulates invasion and DNA synthesis by p38-dependent and p38-independent mechanisms, indicating Ras using distinct pathways to increase breast cancer invasion and growth. Because ER has well-established activities in breast cancer progression (47, 48), we wished next to determine whether ER also regulates invasion and growth through distinct signaling. Previous studies have shown that ER suppresses breast cancer invasion by estrogen-dependent and estrogen-independent mechanisms (13), whereas estrogen can inhibit its own receptor expression (11). Consequently, experiments were done in normal complete medium without estrogen addition to assess effects of ER protein expression.

Results in Fig. 3A and B showed that Tet induces a similar level of ER and ER/T311A protein expression, but ER transcription activity (ERE-Luc, ref. 38) decreases about 90% (P < 0.01) in mutant ER expressed cells. These results are consistent with the previous observation in endometrial adenocarcinoma cells (39). ER expression inhibited invasion >80% (P < 0.01), whereas the mutant ER had no substantial effects (P > 0.05, Fig. 3C, left). A similar result was also obtained when crystal violet–stained cells were quantitated at 600 nm (ref. 42; Fig. 3C, right). Although ER has well-established invasion-inhibitory activity (12, 13), these results suggest that ER may do so through transcriptional regulations. In contrast to the effects on cell invasion, ER and ER/T311A increased DNA synthesis similarly (P > 0.05; Fig. 3D), indicating that ER regulates invasion and DNA synthesis by distinct mechanisms. These results together show that both Ras and ER regulate breast cancer growth and invasion by distinct signal transduction pathways.

View larger version (21K): [in this window] [in a new window]   Figure 3. ER inhibits invasion and stimulates growth by distinct mechanisms. A, ER protein expression in Tet-on cells. Tet-on 231 cells were incubated with and without Tet for 24 hours and examined for ER and ER/T311A protein expression. B, Thr311 is required for ER transcription activity. Cells were transfected with ERE-Luc, incubated with and without Tet for 24 hours, and assessed for luciferase activity. Columns, mean of five independent experiments; bars, SD. C, ER requires its transcription activity to inhibit invasion. Cells were cultured ± Tet for 22 hours in the invasion chamber for the assay (see Materials and Methods). Columns, mean from 16 fields in one experiment; bars, SD. Similar results were obtained in two additional experiments. The absorption at A600 nm (OD600) is mean of three separate experiments. D, ER does not require its transcription activity to stimulate DNA synthesis. Cells were cultured for 24 hours with or without Tet and cell growth was estimated by thymidine incorporation.

ER requires its nuclear localization to bind to p38 protein, leading to its specific down-regulation in the nuclear compartment.

Consistent with previous findings (39), immunostaining analyses showed that ER is mostly localized in the nucleus, whereas ER/T311A is predominantly in the area surrounding the nuclei after a 24-hour incubation with Tet (Fig. 4A ). p38 signals are detected in the nucleus and cytoplasm in ER^– cells. In ER-expressed cells, however, the nuclear p38 signal seems negatively correlating with the ER intensity, indicating that nuclear ER is able to disrupt nuclear p38 protein, leading to its down-regulation in the nuclear compartment. This conclusion is further supported by the observation in ER/T311A cells in which the mutant ER is mostly outside the nucleus and in which there is no decrease in nuclear p38 signals (Fig. 4A).

View larger version (58K): [in this window] [in a new window]   Figure 4. ER antagonizes nuclear p38 activity through direct binding. A, ER is nuclear while ER/T311A is predominantly cytoplasmic. Cells were incubated for 24 hours (±Tet) and double stained for ER (detected with Cy3-labeled second antibody) and for p38 expression (detected with FITC-labeled second antibody) with 4',6-diamidino-2-phenylindole (DAPI) staining as a control for nuclear signals. B, ER disrupts nuclear p38 protein through Thr311-dependent binding. Cells were prepared for nuclear and cytoplasmic fractions, which were analyzed for protein expression (top). p38 binding activity of ER was assessed by immunoprecipitation with a p38 antibody followed by Western analyses (middle). For pulldown assays (bottom), the purified GST, GST-ER, and GST-ER/T311A proteins were incubated with equal amounts of lysates prepared from 293T cells transfected with flag-p38 and flag-p38/AGF, and the precipitates were analyzed for p38-bound ER protein. C, overexpressed p38 is cytoplasmic in ER+ cells. ER+ 231 cells (Tet-on cells incubated with Tet for 24 hours) were infected with Ad-Vect (Vect) or Ad-p38 for 24 hours and stained with anti-flag antibody for transfected flag-p38. D, higher levels of p38 proteins increase invasion (right) but not DNA synthesis (left) in ER+ breast cancer cells. Tet-on 231 cells were plated for invasion and thymidine incorporation after infection. Right, columns, mean from 18 fields of one representative experiment; bars, SD. Similar results were obtained from one additional experiment. Left, columns, mean of four experiments; bars, SD.

To determine whether there is a physical interaction between ER and p38, thereby leading to p38 down-regulation, immunoprecipitation and Western analyses were done. Results in Fig. 4B (middle) show that p38 binds to ER but not ER/T311A, although both proteins are expressed to a similar level from the input control, indicating ER requiring Thr³¹¹ to bind to p38 protein. To further show whether p38 requires its phosphorylation to bind to ER, flag-tagged p38 and its nonphosphorable mutant (p38/AGF) were expressed in 293T cells. Lysates derived were incubated with bacterially expressed GST, GST-ER, GST-ER/T311A proteins, and flag precipitates were examined for bound ER proteins. Results in Fig. 4B (bottom) show that ER, but not ER/T311A, binds to both p38 and p38/AGF proteins, indicating that the direct ER-p38 binding requires ER Thr³¹¹ but not p38 phosphorylation. Together with the immunostaining and cell fractionation analysis, these results show that ER requires its nuclear localization to bind and thereby to disrupt nuclear p38 protein.

p38 overexpression increases invasion but not DNA synthesis in ER⁺ breast cancer cells. Results of ER-inhibiting p38 expression and p38-stimulating ER^– cell invasion suggest that p38 may act downstream of ER to increase invasion. If this is the case, forced p38 expression in ER⁺ cells should overcome this genetic restriction and lead to an invasive response. To relate invasion-regulatory effects with cellular localizations, flag-p38 was overexpressed in ER⁺ cells (Tet-on), and its cellular distributions and activities on invasion were determined. Results in Fig. 4C show that in contrast to the endogenous p38 protein, overexpressed p38 is mostly in the cytoplasm, an effect similar to a recent observation in which overexpressed MK2 leads to its own relocalization (53). Although mechanisms are unclear at present, the cytoplasmic localization of exogenous p38 proteins in ER expressed cells further supports the notion that ER antagonizes nuclear p38 activity, leading to a reduced nuclear p38 concentration even under overexpressed conditions. In the cytoplasm, transfected p38 may have escaped the nuclear ER targeting as a result of their different localizations. As expected, overexpressed p38 led to an increased invasion (3.7-fold) but not thymidine incorporation in these ER⁺ cells (Fig. 4D). These results, thus, further establish the p38-antagonizing activity of ER within the nuclear compartment and reveal that elevation of p38 protein concentrations by forced expression can also increase ER⁺ cell invasion.

ER negatively regulates p38 gene expression in a panel of human breast cancer cell lines. ER-inhibiting p38 protein expression dependent of ERE activity suggests that this regulation may be transcriptional. We would like next to determine if ER antagonizes p38 at RNA levels to further establish the trans-suppression mechanism. Total RNA in this case was prepared from Tet-on cells and analyzed for p38 RNA expression (41) by including p38 as a control. As shown in Fig. 5A (left) , Tet-induced ER decreases p38 but not p38 RNA expression, thereby consolidating our conclusion of ER trans-suppressing p38 expression. To show if this trans-suppression is a general phenomenon, a panel of natural ER⁺ and ER^– breast cancer cell lines were analyzed for p38 RNA expression. ER protein expression has been previously confirmed in ER⁺ MCF-7 and T47D but not in ER^– 231 and 468 human breast cancer cells by Western analyses (40). Consistent with Tet-induced ER expression, higher levels of p38 RNA were detected in ER^– than in ER⁺ cells (Fig. 5A, right), ruling out cell type–specific effects of the p38 antagonistic activity.

View larger version (24K): [in this window] [in a new window]   Figure 5. ER negatively regulates p38 expression in a panel of human breast cancer cell lines. A, ER+ phenotype correlates with lower levels of p38 RNA expression. Total RNA was prepared, separated, and transferred to a nitrocellulose membrane that was hybridized with a specific radioactive-labeled probe for p38 expression. B, ER depletion increases p38 expression. ER+ cells were infected with pSR-Lucif (Lucif) or pSR-siER (siER) for 24 hours and examined for p38 RNA (left) or protein (right) expression. C, ER negatively regulates p38 expression by ligand-independent mechanisms. Cells in steroid-depleted medium were incubated for 24 hours (±10 nmol/L E2) after the pSR infection (left) or in the presence or absence of Tet (right) and analyzed by Western analysis for protein expression.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

 
Uncontrolled proliferation and increased invasion are key characteristics of human cancer, and dissecting these two events is consequently critical for understanding and controlling malignant progression (1). Here, we showed that Ras increases breast cancer invasion and DNA synthesis by p38-dependent and p38-independent pathways. A specific role of p38 in increasing invasion independent of growth was shown by both its depletion and overexpression. Moreover, we provide evidence indicating that ER also inhibits invasion and increases DNA synthesis by distinct pathways, where p38 is specifically involved in regulating cell invasion. These results together show that there exist distinct signal transduction pathways for both Ras and ER to regulate breast cancer invasion and growth in which p38 specifically integrates their antagonistic activity to stimulate invasion (Fig. 6 ). Because invasion is a major characteristic of tumor but not normal cells (1), inhibiting p38-dependent invasive pathways may be a novel strategy to control breast cancer progression.

View larger version (15K): [in this window] [in a new window]   Figure 6. An experimental model illustrates that ER and Ras regulate breast cancer progression through distinct invasive and proliferative pathways where p38 only integrates their antagonistic activity to increase invasion. ER requires transcription activity to suppress Ras/p38 expression and to bind p38 protein, whereas it increases DNA synthesis by ERE-independent mechanisms. Ras, on the other hand, increases invasion and DNA synthesis through p38-dependent and p38-independent pathways in ER– cells. Although loss of ER expression may reduce cell growth, resultant Ras activation will provide mitogenic signaling, leading to increased DNA synthesis [and possible cell proliferation (?)]. Induced p38 following ER inactivation and/or Ras activation will specifically mediate Ras nonmitogenic signaling to stimulate invasion. Through these two mechanisms, Ras/p38 activation will lead to an increased breast cancer progression. This model suggests a feasibility to individually target invasive and proliferative signal transduction pathways in human breast cancers.

The central mechanism by which ER antagonizes the Ras/p38 activity is likely through its nuclear localization that integrates transcriptional and posttranscriptional regulatory processes. This was shown by the fact that inhibition of ER nuclear localization through Thr³¹¹ mutation both reduces ERE-dependent transcription and disrupts its p38 binding activity. These results are consistent with the notion that nuclear localization is essential for activities of nuclear receptors (55). Although a decreased ERE by ER/T311A correlating with the loss of p38 binding activity suggests a role of this interaction in ER transcription, a decreased p38 expression in ER⁺ breast cancer cells may argue against its physiologic roles in regulating ER nuclear localization and ER activity. Additional studies, however, are needed to explore mechanisms by which the ER direct binding leads to a p38 down-regulation in the nuclear compartments.

Our results may offer an explanation about paradoxical ER effects in stimulating growth and in inhibiting invasion, which may otherwise antagonize each other in regulating breast cancer progression. Although loss of ER expression may reduce breast cancer growth, the resultant Ras activation can compensate for this effect by a proliferative response through increased expression (Fig. 6). This theory is supported by the observation of higher levels of Ras protein expression in ER^– and/or metastatic human breast cancers (19, 44, 54, 56, 57). Because ER inactivation and Ras activation frequently occur in late stage of the disease (54, 56), these results may suggest a stage-specific role of ER and Ras in promoting breast cancer progression through a coordinative signaling integration.

It is well accepted that Ras uses distinct effector pathways to induce malignant transformation/progression (2, 46, 58). Our studies here are the first to show the existence of such pathways under physiologic conditions in which induced p38 transmits Ras nonmitogenic signaling to amplify its invasion signals without affecting its proliferative activity. This specific pathway was first suggested by positive regulation of p38 expression through Ras activation and inactivation, then confirmed by ER inhibiting both Ras and p38 expression, and finally proven by p38-mediated rescue of N17-induced invasion inhibition. Although ERK and/or p38 phosphorylations are involved in regulating breast cancer invasion (26, 42), these effects could be secondary to altered cell proliferation. Here, we show that Ras dictates p38 expression without affecting ERK/p38 phosphorylation in human breast cancer, and p38 in turn increases invasion without affecting Ras mitogenic activity. These results together suggest that p38 act as a Ras effector to stimulate invasion in response to ER inactivation/Ras activation.

	Acknowledgments

 
Grant support: NIH grant 2R01 CA91576 and Department of Veterans Affairs Merit Review (G. Chen).

The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

We thank Melanine Weytkow for assistance in some experiments and Drs. Jiahuai Han (The Scripps Research Institute, La Jolla, CA), Dennis Stacey (The Cleveland Clinic Foundation, Cleveland, OH), David Shapiro (University of Illinois, Urbana, IL), and Dan Mercola (Sidney Kimmel Cancer Center, San Diego, CA) for providing reagents.

Received 12/29/05. Revised 4/20/06. Accepted 6/ 2/06.

	References

Top Abstract Introduction Materials and Methods Results Discussion References

 

1. Hanahan D, Weiberg RA. The hallmarks of cancer. Cell 2000;100:57–70.[CrossRef][Medline]
2. Campbell PM, Der CJ. Oncogenic Ras and its role in tumor cell invasion and metastasis. Semin Cancer Biol 2004;14:105–14.[CrossRef][Medline]
3. Gao CF, Xie Q, Su YL, et al. Proliferation and invasion: plasticity in tumor cells. Pro Natl Acad Sci U S A 2005;102:10528–33.[Abstract/Free Full Text]
4. Oft M, Akhurst RJ, Balmain A. Metastasis is driven by sequential elevation of H-ras and Smad2 levels. Nat Cell Biol 2002;4:487–94.[CrossRef][Medline]
5. Huntington JT, Shields JM, Der CJ. et al. Overexpression of collagenase 1 (MMP-1) is mediated by the ERK pathway in invasive melanoma cells. Role of b-raf mutation and fibroblast growth factor signaling. J Biol Chem 2004;279:33168–76.[Abstract/Free Full Text]
6. Scott LA, Vass JK, Parkinson EK, Gillespie DAF, Winnie JN, Ozanne BW. Invasion of normal human fibroblasts induced by v-Fos is independent of proliferation, immortalization, and the tumor suppressors p16^INK4a and p53. Mol Cell Biol 2004;24:1540–59.[Abstract/Free Full Text]
7. Joneson T, White MA, Wigler MH, Bar-Sagi D. Stimulation of membrane ruffling and MAP kinase activation by distinct effectors of Ras. Science 1996;271:810–2.[Abstract]
8. Roderiguez-Viciana P, Warne PH, Khwaja A, et al. Role of phosphoinositide 3-OH kinase in cell transformation and control of the actin cytoskeleton by Ras. Cell 1997;89:457–67.[CrossRef][Medline]
9. Downward J. Targeting Ras signalling pathways in cancer therapy. Nat Rev Cancer 2003;3:11–22.[CrossRef][Medline]
10. Fujita T, Kobayashi Y, Wada O, et al. Full activation of estrogen receptor a activation function-1 induces proliferation of breast cancer cells. J Biol Chem 2003;278:26704–14.[Abstract/Free Full Text]
11. Pinzone JJ, Stevenson H, Stroble J, Berg PE. Molecular and cellular determinants of estrogen receptor expression. Mol Cell Biol 2004;24:4605–12.[Free Full Text]
12. Garcia M, Deroco D, Freiss G, Rochefort H. Activation of estrogen receptor transfected into a receptor-negative breast cancer cell line decreases the metastatic and invasive potential of the cells. Pro Natl Acad Sci U S A 1992;89:11538–42.[Abstract/Free Full Text]
13. Platet N, Cunat S, Chalbos D, Rochefort H, Garcia M. Unliganded and liganded estrogen receptors protect against cancer invasion via different mechanisms. Mol Endocrinol 2000;14:999–1009.[Abstract/Free Full Text]
14. Clark R, Thompson EW, Leonessa F, et al. Hormone resistance, invasiveness and metastatic potential in breast cancer. Breast Cancer Res Treat 1993;24:227–39.[CrossRef][Medline]
15. Van't Veer LJ, Dai H, Van de Vijver MJ, et al. Gene expression profiling predicts clinical outcome of breast cancer. Nature 2002;415:530–6.[CrossRef][Medline]
16. Janda E, Lehmann K, Killisch I, et al. Ras and TGFß cooperatively regulate epithelial cell plasticity and metastasis: dissection of Ras signaling pathways. J Cell Biol 2002;156:299–313.[Abstract/Free Full Text]
17. Kasid A, Lippman ME, Papageorge AG, Lowy DR, Gelmann EP. Transfection of v-ras^H DNA into MCF-7 human breast cancer cells bypasses dependence on estrogen for tumorigenicity. Science 1985;228:725–8.[Abstract/Free Full Text]
18. deFazio A, Chiew YE, McEvoy M, Watts CK, Sutherland RL. Antisense estrogen receptor RNA expression increases epidermal growth factor receptor gene expression in breast cancer cells. Cell Growth Differ 1997;8:903–11.[Abstract]
19. Rundle A, Tang D, Brand-Rauf P, et al. Association between the ras p21 oncoprotein in blood samples and breast cancer. Cancer Lett 2002;185:71–8.[CrossRef][Medline]
20. Ozer E, Sis B, Ozen E, Sakizli M, Canda T, Sarioglu S. BRCA1, C-erbB-2, and H-ras gene expression in young women with breast cancer. An immunohistochemical study. App Imm Mol Morphol 2000;8:12–8.
21. Mansour S, Matten WT, Hermann AS, et al. Transformation of mammalian cells by constitutively active MAP kinase kinase. Science 1994;265:966–70.[Abstract/Free Full Text]
22. Cowley S, Paterson H, Kemp P, Marshall CJ. Activation of MAP kinase is necessary and sufficient for PC12 differentiation and for transformation of NIH 3T3 cells. Cell 1994;77:841–52.[CrossRef][Medline]
23. Chen G, Hitomi M, Han J, Stacey DW. The p38 pathway provides negative feedback to Ras proliferative signaling. J Biol Chem 2000;275:38973–80.[Abstract/Free Full Text]
24. Qi X, Tang J, Pramanik R, et al. p38 MAPK activation selectively induces cell death in K-ras mutated human colon cancer cells through regulation of vitamin D receptor. J Biol Chem 2004;279:22138–44.[Abstract/Free Full Text]
25. Bulavin DV, Phillips C, Nannenga B, et al. Inactivation of the Wip1 phosphatase inhibits mammary tumorigenesis through p38 MAPK-mediated activation of the p16Ink4a-p19Arf pathway. Nat Genet 2004;36:343–50.[CrossRef][Medline]
26. Kim MS, Lee EJ, Kim HRC, Moon A. p38 kinase is a key molecule for H-Ras-induced cell motility and invasive phenotype in human breast epithelial cells. Cancer Res 2003;63:5454–61.[Abstract/Free Full Text]
27. Pramanik R, Qi X, Borowicz S, et al. p38 isoforms have opposite effects on AP-1-dependent transcription through regulation of c-Jun: the determinant role of the isoforms in the p38 MAPK signal specificity. J Biol Chem 2003;278:4831–9.[Abstract/Free Full Text]
28. Wang L, Ma R, Flavell R, Choi ME. Requirement of mitogen-activated protein kinase kinase 3 (MKK3) for activation of p38 and p38 MAPK isoforms by TGF-ß1 in murine mesangial cells. J Biol Chem 2002;277:42257–62.
29. Ono K, Han J. The p38 signal transduction pathway. Activation and function. Cell Signal 2000;12:1–13.[CrossRef][Medline]
30. Lechner C, Zahalka MA, Giot J, Moller NP, Ullrich A. ERK6, a mitogen-activated protein kinase involved in C2C12 myoblast differentiation. Pro Natl Acad Sci U S A 1996;93:4355–9.[Abstract/Free Full Text]
31. Li Z, Jiang Y, Ulevitch RJ, Han J. The primary structure of p38g: a new member of p38 group of MAP kinases. Biochem Biophys Res Commun 1996;228:334–40.[CrossRef][Medline]
32. Wang X, McGowan CH, Zhao M, et al. Involvement of the MKK6-38 cascade in -radiation-induced cell cycle arrest. Mol Cell Biol 2000;20:4543–52.[Abstract/Free Full Text]
33. Abdollahi T, Robertson NM, Abdollahi A, Litwack G. Identification of interleukin 8 as an inhibitor of tumor necrosis factor-related apoptosis-inducing ligand-induced apoptosis in the ovarian carcinoma cell line OVCAR3. Cancer Res 2003;63:4521–6.[Abstract/Free Full Text]
34. Tang J, Qi X, Mercola D, Han J, Chen G. Essential role of p38 in K-Ras transformation independent of phosphorylation. J Biol Chem 2005;280:23910–7.[Abstract/Free Full Text]
35. Shu J, Lee JH, Harwalka JA, Oh-Siskovic S, Stacey DW, Golubic M. Adenovirus-mediated gene transfer of dominant negative Ha-Ras inhibits proliferation of primary meningioma cells. Neurosurgery 1999;44:579–88.[CrossRef][Medline]
36. Hayakawa J, Depatie C, Ohmichi M, Mercola D. The activation of c-Jun NH2-terminal kinase (JNK) by DNA-damaging agents serves to promote drug resistance via activating transcription factor 2 (ATF2)-dependent enhanced DNA repair. J Biol Chem 2003;278:20582–92.[Abstract/Free Full Text]
37. Brummelkamp TR, Bernards R, Agami R. A system for stable expression of short interfering RNAs in mammalian cells. Science 2002;296:550–3.[Abstract/Free Full Text]
38. Zhang CC, Shapiro DJ. Activation of the p38 mitogen-activated protein kinase pathway by estrogen or by 4-hydroxytamoxifen is coupled to estrogen receptor-induced apoptosis. J Biol Chem 2000;275:479–86.[Abstract/Free Full Text]
39. Lee H, Bai W. Regulation of estrogen receptor nuclear export by ligand-induced and p38-mediated receptor phosphorylation. Mol Cell Biol 2002;22:5835–45.[Abstract/Free Full Text]
40. Qi X, Borowicz S, Pramanik R, Schultz RM, Han J, Chen G. Estrogen receptor inhibits c-Jun-dependent stress-induced cell death by binding and modifying c-Jun activity in human breast cancer cells. J Biol Chem 2004;279:6769–77.[Abstract/Free Full Text]
41. Qi X, Pramank R, Wang J, et al. The p38 and JNK pathways cooperate to trans-activate vitamin D receptor via AP-1 and sensitize human breast cancer cells to vitamin D3-induced growth inhibition. J Biol Chem 2002;277:25884–92.[Abstract/Free Full Text]
42. Huang S, New L, Pan Z, Han J, Nemerow GR. Urokinase plasminogen activator/urokinase-specific surface receptor expression and matrix invasion by breast cancer cells requires constitutive p38 mitogen-activated protein kinase activity. J Biol Chem 2000;275:12266–72.[Abstract/Free Full Text]
43. Asada M, Yamada T, Ichijo H, et al. Apoptosis inhibitory activity of cytoplasmic p21^cip/WAF1 in monocytic differentiation. EMBO J 1999;8:1223–34.[CrossRef]
44. Eckert LB, Repasky GA, Ulku AS, et al. Involvement of Ras activation in human breast cancer signaling, invasion, and anoikis. Cancer Res 2004;64:4585–92.[Abstract/Free Full Text]
45. Sommers CL, Papageorge AG, Wilding G, Gelmann EP. Growth properties and tumorigenesis of MCF-7 cells transfected with isogenic mutants of ras^H. Cancer Res 1990;50:67–71.[Abstract/Free Full Text]
46. Marshall CJ. Ras effectors. Curr Opin Cell Biol 1996;8:197–204.[CrossRef][Medline]
47. Platet N, Cathiard AM, Gleizes M, Garcia M. Estrogen and their receptors in breast cancer progression: a dual role in cancer proliferation and invasion. Crit Rev Oncol Hematol 2004;51:55–67.[Medline]
48. Oesterreich S, Zhang P, Guler RL, et al. Re-expression of estrogen receptor in estrogen -negative MCF-7 cells restores both estrogen and insulin-like growth factor-mediated signaling and growth. Cancer Res 2001;61:5771–7.[Abstract/Free Full Text]
49. Sabio G, Simon J, Arthur C, et al. p38 regulates the localisation of SAP97 in the cytoskeleton by modulating its interaction with GKAP. EMBO J 2005;24:1134–45.[CrossRef][Medline]
50. Lawrence T, Beblen M, Liu GY, Nizet V, Karin M. IKK limits macrophage NF-kB activation and contributes to the resolution of inflammation. Nature 2005;434:1138–43.[CrossRef][Medline]
51. New L, Jiang Y, Han J. Regulation of PRAK subcellular location by p38 MAP kinases. Mol Biol Cell 2003;14:2603–16.[Abstract/Free Full Text]
52. Piotrowicz RS, Ding L, Maher P, Levin EG. Inhibition of cell migration by 24-kDa fibroblast growth factor-2 is dependent upon the estrogen receptor. J Biol Chem 2001;276:3963–70.[Abstract/Free Full Text]
53. Seternes O, Mikalsen T, Johansen B, et al. Activation of MK5/PRAK by the atypical MAP kinase ERK3 defines a novel signal transduction pathway. EMBO J 2004;23:4780–91.[CrossRef][Medline]
54. von Lintig FC, Dreilinger AD, Varki NM, Wallace AM, Casteel DE, Boss GR. Ras activation in human breast cancer. Breast Cancer Res Treat 2000;62:51–62.[CrossRef][Medline]
55. Hall JM, Couse JF, Korach KS. The multifaceted mechanisms of estradiol and estrogen receptor signaling. J Biol Chem 2001;276:36869–72.[Free Full Text]
56. Lundy J, Grimson R, Mishriki Y, Chao S, Ovarez S, Fromowitz F. Elevated ras oncogene expression correlates with lymph node metastases in breast cancer patients. J Clin Oncol 1986;4:1321–5.[Abstract/Free Full Text]
57. Clair T, Miller W, Cho-Chung Y. Prognostic significance of the expression of the ras protein with a molecular weight of 21,000 by human breast cancer. Cancer Res 1987;47:5290–3.[Abstract/Free Full Text]
58. Malumbres M, Barbacid M. Ras oncogenes: the first 30 years. Nat Rev Cancer 2003;3:7–13.[CrossRef]

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