From the
Department of Cell and Cancer Biology,
NCI, National Institutes of Health, Rockville, Maryland 20850-3300, the
Department of Pharmacology, University of North
Carolina, Chapel Hill, North Carolina 27599-7295, and
¶The Center for Cancer Research, NCI, National
Institutes of Health, Bethesda, Maryland 20892
Received for publication, January 17, 2003 , and in revised form, May 2, 2003.
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ABSTRACT |
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INTRODUCTION |
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RASSF1 has recently been identified as a potential tumor suppressor that can serve as a Ras effector (12, 13). RASSF1 can induce apoptosis or cell cycle arrest (12, 14) and is frequently down-regulated by promoter methylation during tumorigenesis (15). NORE1 is related to RASSF1 and can also induce a Ras-dependent apoptosis (16, 17). Like RASSF1, NORE1 is frequently down-regulated in primary tumors and tumor cell lines (17). Data base analysis suggests that there may be more members of this family. We identified in the GenBankTM data base a human RASSF1-like hypothetical protein that was originally designated KIAA0168 but now is being referred to as RASSF2. We cloned the gene and sought to determine whether RASSF2 is also a Ras effector/tumor suppressor of the RASSF1 family.
We now report that RASSF2 can bind directly to K-Ras in a GTP-dependent manner via the Ras effector domain. Therefore, RASSF2 demonstrates the basic characteristics of a Ras effector. The interaction of RASSF2 with Ras appears to be specific to K-Ras, as only a weak interaction could be detected with H-Ras.
Rather than promoting transformation, over-expression of RASSF2 inhibits the growth of lung tumor cells. RASSF2-mediated growth inhibition is enhanced by activated K-Ras and appears to involve both apoptosis and cell cycle arrest. Analysis of RASSF2 protein expression in a series of human lung tumor cell lines shows that the protein is frequently down-regulated. Thus, we show that RASSF2 is a new member of the RASSF1 family and shares the properties of being a potential Ras effector/tumor suppressor.
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MATERIALS AND METHODS |
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DNA and PlasmidsRASSF2 was identified as IMAGE Consortium clone 22950 distributed by the American Type Culture Collection (ATCC; Manassas, VA). The RASSF2 coding region was PCR-cloned using oligomers 5'-ggatccatggactacagccaccaaac and 3'-caattgtcagattgttgctggggtc, which added a BamHI site to the 5' end and an MfeI site to the 3' end. After sequencing to confirm fidelity, the gene was cloned into pZIPHA, pCDNAF (17), and pEGFP (Clontech, Palo Alto, CA) as a BamHI/MfeI fragment. The RA domain of RASSF2 (nucleotides 535789) was cloned as a BamHI/MfeI fragment into pMal (New England BioLabs, Beverly, MA) and pGEX2T (Amersham Biosciences). Activated K-Ras was cloned into the BamHI site of pCGNHA (19), and effector mutants were generated using a QuikChange kit (Stratagene, La Jolla, CA).
Ras Binding AssaysIn vivo assays were performed by transfecting 293-T cells with 5 µg of each plasmid using LipofectAMINE 2000 (Invitrogen). After 48 h, the cells were lysed in modified radioimmune precipitation assay buffer (20) and immunoprecipitated with HA beads (Sigma). The immunoprecipitate was then subjected to Western analysis with an anti-FLAG monoclonal (Sigma) to measure the co-precipitation of RASSF2. In vitro binding assays were performed using purified GST fusion protein of the RA domain of RASSF2 and purified K-Ras derived from baculovirus-infected Sf9 cells (a generous gift of D. Stokoe, University of California, San Francisco, CA). K-Ras protein was loaded with the GTP analog guanylyl-5-imidodiphosphate (Sigma) by incubating in 100 mM Tris, pH 8, 50 mM NaCl, and 10 mM EDTA with 6 mM GTP analog (Sigma) for 10 min at room temperature. The loaded protein was then stabilized with 10 mM MgCl2. 2 pg of loaded protein were then added to 100 ng of fusion protein on Sepharose beads in phosphate-buffered saline with 1x protease inhibitors (Pharmingen), 5 mM MgCl2, 1 µM ZnCl2, and 0.01% Tween 20. The proteins were rotated at 4 °C for 1 h, washed three times, and then subjected to Western analysis.
Growth Inhibition AssaysCell lines were obtained from the ATCC. A549 human lung carcinoma cells were transfected with 1 µg of pZIPHA RASSF2 or empty vector and selected in 500 µg/ml of G418 (Invitrogen) for 2 weeks. Cells were fixed and stained with crystal violet. Transient growth inhibition assays were performed in 293-T cells by transfecting with LipofectAMINE 2000 (Invitrogen) as described previously (12).
Apoptosis AssaysRASSF2-induced apoptosis was examined by using the pCaspase3-Sensor system (Clontech) and fluorescent microscopy to measure caspase-3 activation in individual live cells. This system uses an enhanced yellow fluorescent protein (EYFP) fused with a nuclear export signal and a nuclear localization signal. The nuclear export signal is dominant and separated from the EYFP by a caspase-3 cleavage site. In the absence of active caspase-3, the EYFP localizes to the cytosol. In the presence of active caspase-3, the nuclear export signal is cleaved off, and the nuclear localization signal promotes transport into the nucleus. Cells were transfected with 100 ng of pCaspase3-Sensor and/or red fluorescent protein-RASSF2. After 24 h, red cells were examined for the localization of EYFP. The detection of caspase-3 activation and induction of apoptosis using this method were quantified by identifying and counting cells that co-expressed the nuclear localized pCaspase3-Sensor protein and red fluorescent protein-RASSF2.
In situ trypan blue uptake was performed on 293 HEK cells (ATCC). Cells were transfected with 5 µg of RASSF2 in the presence or absence of 50 ng of K-Ras12V. 72 h post-transfection trypan blue was added at a final concentration of 0.04%. Dye uptake was quantitated by counting the number of blue cells in three random 40x fields.
Fluorescence-activated Cell Sorting AnalysisCell cycle analysis was performed in 293-T cells transfected with 5 µg of pEGFP empty vector or pEGFP-RASSF2 using LipofectAMINE 2000 (Invitrogen). 24 h after transfection cells were harvested and resuspended at a concentration of 2 x 106 cells/ml in medium with low serum (2%). Hoechst 33342 (Sigma) was added to a final concentration of 3 µg/ml and incubated for 1 h at 37 °C. After incubation cells were immediately centrifuged in the cold, resuspended to a final concentration of 1 x 106 cells/ml, and subjected to fluorescence-activated cell sorting analysis. DNA content of GFP-positive cells was determined using a fluorescence-activated cell sorting Vantage S.E. (BD Biosciences). The software programs CellQuest (BD Biosciences) and ModFit (Verity Software House) were used for data acquisition and cell cycle modeling.
Northern AnalysisA commercial, prequantitated normal tissue blot of mRNA was obtained from Clontech. The coding region of RASSF2 was used as a probe. Experiments were performed as described previously (12).
Assay of RASSF2 Protein Expression in Tumor Cell LinesRASSF2 polyclonal antiserum was prepared to the peptide GLRRPIRLQMQDDNERIR (residues 6178) by ResGen (Huntsville, AL) and affinity-purified. The antibody did not cross-react with NORE1 or RASSF1 (data not shown). Specificity was confirmed by peptide competition experiments (data not shown). The antibody was then used at a dilution of 1/1000 to perform Western analysis of a series of human lung tumor cell lines.
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RESULTS |
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Binding of K-Ras to RASSF2To determine whether Ras and RASSF2 could interact, we first performed co-transfection experiments in 293-T cells with FLAG-tagged RASSF2 and HA-tagged activated and wild type K-Ras. After 48 h, cells were lysed and immunoprecipitated with HA-Sepharose beads (Sigma) for 1 h. After washing, the immunoprecipitate was subjected to Western analysis using an anti-FLAG antibody. Fig. 2a (top) shows that RASSF2 preferentially precipitates with activated K-Ras. The relative quantities of Ras and RASSF2 in the lysate were determined by immunoblotting the lysate with HA and FLAG (Fig. 2a, bottom). We next determined if the interaction required the effector domain of Ras by using a similar strategy with a series of effector mutants of K-Ras. Figure 2b (top) shows that mutations in the effector domain of K-Ras severely impair the ability of the protein to bind RASSF2. Again, a Western blot of the lysates before immunoprecipitation is shown at the bottom of Fig. 2b. Finally, we examined the possibility that RASSF2 might preferentially bind K-Ras over H-Ras. In Fig. 2c we show that although activated K-Ras readily precipitated RASSF2, the levels of RASSF2 precipitating with activated H-Ras were barely detectable. Protein levels in the lysate are again shown at the bottom of Fig. 2c.
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To confirm that the K-Ras-RASSF2 interaction is direct, we prepared recombinant GST fusion protein of the RA domain of RASSF2. This was used as an affinity reagent to precipitate purified, farnesylated K-Ras (generous gift of D. Stokoe, University of California, San Francisco, CA). Fig. 3a shows that the RASSF2-RA domain fusion protein can precipitate farnesylated K-Ras from solution. Equal loading of GST fusion protein was confirmed by Western blotting of a sample of the precipitate with an anti-GST antibody (Fig. 3b) (Santa Cruz Biochemicals, Santa Cruz, CA). Note that the GST-RA domain fusion protein construct also produced GST. Similar results were obtained with a maltose-binding protein fusion of the RASSF2 RA domain (data not shown). Therefore, RASSF2 binds directly to K-Ras in a GTP-dependent manner via the effector domain.
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RASSF2 Expression Inhibits Cell GrowthRASSF2 was cloned into a selectable expression vector, pZIPHA, and transfected into A549 human lung carcinoma cells. Cells were selected for 2 weeks and then stained with crystal violet (Fig. 4). Cells transfected with RASSF2 failed to generate colonies, whereas the vector alone gave a virtually confluent plate.
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As we were unable to generate stable cell lines expressing RASSF2, we resorted to transient transfections to determine the effects of Ras on RASSF2-mediated growth inhibition. 293-T cells were transfected with RASSF2 ± activated Ras and examined after 48 h (Fig. 5). At this time point, modest growth inhibition was detected with the RASSF2 alone, but this was dramatically enhanced by the presence of activated K-Ras. Interestingly, H-Ras had little effect on this activity. To determine whether the growth inhibition by RASSF2 was apoptotic in nature and whether the presence of activated Ras enhanced this process, we transfected 293 cells with RASSF2 ± K-Ras12V. 72 h post-transfection we added trypan blue directly to the cells and quantitated dead cells by dye uptake. Fig. 6 shows that RASSF2 on its own promotes modest cell death, but in the presence of activated K-Ras cell death is enhanced. Quantification is shown in Fig. 6b.
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RASSF2 Promotes Apoptosis and Cell Cycle ArrestTo determine the mechanistic basis of the RASSF2-mediated growth inhibition, we used the pCaspase3-Sensor system (Clontech) and fluorescent microscopy to measure caspase-3 activation in individual cells. Cells were co-transfected with pCaspase3-Sensor and red fluorescent protein-RASSF2. After 24 h, red cells were examined for the localization of EYFP. Fig. 7a shows that in vector-transfected cells the EYFP remained cytosolic. However, in RASSF2-co-transfected cells, the majority of cells showed nuclear localization of EYFP, hence demonstrating caspase-3 activation and apoptosis. The results are quantified in Fig. 7b.
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We also performed cell cycle assays on GFP-RASSF2-transfected 293-T cells.
Fig. 8 demonstrates that
GFP-RASSF2-expressing cells consistently show an 20% decrease in the
G2/M phase of the cell cycle, suggesting that the cells tend to
arrest in the G0/G1 phase.
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Expression of RASSF2 in Normal Tissue and Tumor CellsTo determine the tissue specificity of RASSF2 we performed Northern analysis on a commercial normal tissue mRNA blot. A single transcript was detected at 5.4 kb in most tissue. The signal was most intense in the brain, peripheral blood, placenta, and lung samples (Fig. 9). To determine whether RASSF2 might be down-regulated during tumorigenesis, we generated a RASSF2-specific polyclonal antibody. We prepared lysates from a series of human lung tumor cell lines and examined them for RASSF2 protein expression. A normal bronchial epithelial cell line was used as a control. Western analysis demonstrated that the RASSF2 protein was frequently down-regulated in the human lung tumor cell lines (Fig 10). Proliferating cell nuclear antigen was used as an internal control for protein loading.
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DISCUSSION |
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Ras pathways mediating growth inhibition and death are not as well characterized as those used to promote mitogenesis and transformation. However, the recent discovery of the NORE1-RASSF1 class of Ras effectors has started to address this deficiency. RASSF1 and NORE1 have been reported to mediate Ras-dependent apoptosis as well as cell cycle arrest (12, 14, 16, 17). Not only do these proteins mediate growth inhibition, but they are also frequently down-regulated during tumor development. Moreover, reintroduction of the genes into tumor cell lines results in a loss of tumorigenicity (13, 16, 17). Therefore, these proteins have the potential to serve as tumor suppressors that are directly activated by Ras. Loss of function of these growth-inhibitory Ras-controlled pathways may prove as critical as gain of function of conventional Ras-controlled pathways during tumor development. Bioinformatic data base analysis suggests that there may be several other members of the NORE1-RASSF1 family that remain uncharacterized. We have now cloned and characterized RASSF2 to determine whether it too serves as a Ras effector/tumor suppressor.
Examination of the Ras binding properties of RASSF2 showed that it would readily associate with farnesylated K-Ras in a GTP-preferential manner. Moreover, the interaction was direct as the purified RA domain bound purified, farnesylated K-Ras4B. K-ras is the most commonly activated ras gene in human tumors (25) and is the only ras gene that is essential for embryonic development (26). Thus, it appears that K-Ras protein is functionally different from the other Ras isoforms and has a special role in transformation and development. It has been hypothesized that the reason for the special properties of K-Ras is that there may be certain Ras effector proteins that are particularly critical to tumorigenesis and development that preferentially associate with K-Ras (27). However, although differences in effector binding between the Ras isoforms have been reported (28), these involved only a 23-fold difference in binding activity. Here we see an almost complete preference for K-Ras over H-Ras. Thus, RASSF2 could play a key role in mediating some of the unique biological properties of K-Ras.
As we had found some difficulty in showing stable association of RASSF2 with H-Ras, we manufactured the three classic Ras effector mutants, E37G, T35S, and Y40C (29) in K-Ras4B12V. Only the T35S mutant retained any ability to interact with RASSF2, and this was rather weak. Thus, the interaction of RASSF2 and K-Ras4B is via the Ras effector domain. Hence, RASSF2 meets the basic requirements for a potential Ras effector. Ras effector mutants have been used as tools to identify the Ras pathways that are critical for tumor development (30, 31). Interpreting the results of this type of study should now take into account the potential loss of interaction with tumor suppressor effectors, such as RASSF2, as well as the loss of interaction with oncoprotein effectors, such as Raf-1.
The mechanism of action of the RASSF1 family of proteins remains under investigation. Whereas RASSF1 and NORE1 have been shown to promote apoptosis in some cell types (12, 16, 17), Shivakumar et al. (14) suggest they cause cell cycle arrest, not apoptosis, in others. Consequently, we decided to examine both parameters for RASSF2. We found that RASSF2 promoted the activation of caspase-3 in COS-7 cells. A similar effect was observed in 293-T cells (data not shown), but the results were much clearer in the COS-7 cell type due to their flatter morphology. Thus, RASSF2 can promote apoptosis. To examine cell cycle effects, we used fluorescence-activated cell sorting analysis of GFP-RASSF2 expressing 293-T cells. These fast cycling cells showed a 20% decrease in the G2/M component in three separate experiments. This suggests that the cells are tending to arrest in G0/G1. Thus, RASSF2 can promote apoptosis and cell cycle arrest.
A potential mechanism for NORE1-induced apoptosis was recently identified by Khokhlatchev et al. (16) when it was demonstrated that NORE1 binds to the pro-apoptotic kinase MST1. However, they were unable to demonstrate that NORE1 activated the MST1 kinase activity (in fact, it appears to inhibit it), and so although this is an intriguing observation, the role of MST1 kinase in NORE1/RASSF1/RASSF2-mediated cell death remains unclear.
Analysis of RASSF2 mRNA levels in normal tissue shows considerable differential expression. Interestingly, some of the tissues which show the lowest levels of RASSF2 expression (heart, kidney, and skeletal muscle) give among the highest levels of RASSF1 expression in an identical blot (12). Both genes show detectable levels of mRNA in normal lung tissue.
Analysis of RASSF2 expression in a panel of lung tumor cell lines showed that the protein is expressed at modest levels in a normal human bronchial epithelia cell line but fell to undetectable levels in most of the tumor cell lines examined. Intriguingly, one cell line, 441, showed very high levels of RASSF2 expression. This suggests that either there is a mutation in the RASSF2 that renders it non-growth-inhibitory or that there is a mutation in a downstream component of the RASSF2 pathway that makes this cell line resistant to RASSF2-mediated growth inhibition. These possibilities are currently being investigated.
In summary, we now identify a third member of the RASSF1-NORE1 family that preferentially binds K-Ras with the characteristics of an effector. RASSF2 inhibits the growth of tumor cells, and its growth-inhibitory properties are enhanced by activated K-Ras. RASSF2 promotes both cell cycle arrest and apoptosis; consequently, its down-regulation may play a key role in the development of cancer.
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FOOTNOTES |
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|| To whom correspondence should be addressed: Dept. of Cell and Cancer Biology, NCI, National Institutes of Health, 9610 Medical Center Dr., Rockville, MD 20850-3300. Tel.: 301-594-7288; Fax: 301-402-4422; E-mail: gclark{at}mail.nih.gov.
1 The abbreviations used are: RA, Ras association; HA, hemagglutinin; GST,
glutathione S-transferase; EYFP, enhanced yellow fluorescent protein;
GFP, green fluorescent protein.
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REFERENCES |
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