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Tripartite Motif Protein 32 Facilitates Cell Growth and Migration via Degradation of Abl-Interactor 2

Departments of ¹ Biochemistry and ² Otolaryngology, Head and Neck Surgery, Hokkaido University Graduate School of Medicine, Sapporo, Japan

Requests for reprints: Shigetsugu Hatakeyama, Department of Biochemistry, Hokkaido University Graduate School of Medicine, N15, W7, Kita-ku, Sapporo, Hokkaido 060-8638, Japan. Phone: 81-11-706-5899; Fax: 81-11-706-5169; E-mail: hatas{at}med.hokudai.ac.jp.

	Abstract

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Tripartite motif protein 32 (TRIM32) mRNA has been reported to be highly expressed in human head and neck squamous cell carcinoma, but the involvement of TRIM32 in carcinogenesis has not been fully elucidated. In this study, we found by using yeast two-hybrid screening that TRIM32 binds to Abl-interactor 2 (Abi2), which is known as a tumor suppressor and a cell migration inhibitor, and we showed that TRIM32 mediates the ubiquitination of Abi2. Overexpression of TRIM32 promoted degradation of Abi2, resulting in enhancement of cell growth, transforming activity, and cell motility, whereas a dominant-negative mutant of TRIM32 lacking the RING domain inhibited the degradation of Abi2. In addition, we found that TRIM32 suppresses apoptosis induced by cis-diamminedichloroplatinum (II) in HEp2 cell lines. These findings suggest that TRIM32 is a novel oncogene that promotes tumor growth, metastasis, and resistance to anticancer drugs. [Cancer Res 2008;68(14):5572–80]

	Introduction

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Ubiquitination is a versatile posttranslational modification mechanism used by eukaryotic cells mainly to control protein levels through proteasome-mediated proteolysis. Ubiquitin conjugation is achieved by several enzymes that act in concert, including a ubiquitin-activating enzyme (E1), a ubiquitin-conjugating enzyme (E2), and a ubiquitin-protein ligase (E3; refs. 1, 2). E3 is thought to be the component of the ubiquitin conjugation system that is most directly responsible for substrate recognition. Enzymes belonging to class E3 that have thus far been identified include members of the HECT (homologous to E6-AP carboxyl terminus), RING-finger, and U-box families of proteins (3–5).

Tripartite motif (TRIM) proteins are characterized by the presence of a RING finger, one or two zinc-binding motifs named B-boxes, and an associated coiled-coil region (6). Most TRIM proteins have been reported to have a role in the ubiquitination process, for example, TRIM25 (EFP) ubiquitinates 14-3-3 (7), estrogen receptor (8), and retinoic acid–inducible gene I (9). Furthermore, several TRIM family members are involved in various cellular processes, such as transcriptional regulation, cell growth, apoptosis, development, and oncogenesis (10–12).

The TRIM family protein TRIM32 was identified as a protein that interacts with the activation domain of lentiviral Tat proteins (activators of viral transcription; ref. 13). Each TRIM family member is characterized by a specific carboxyl-terminal domain (6). TRIM32 contains six repeats of the NHL (NCL-1, HT2A, and LIN-41) motif, which is likely to mediate protein-protein interactions (14). Point mutations of human TRIM32 have been reported in two autosomal recessive genetic disorders: limb-girdle muscular dystrophy type 2H, which is a myopathy with a primary or predominant involvement of the pelvic or shoulder girdle musculature (15), and Bardet-Biedl syndrome, which is characterized by obesity, pigmentary retinopathy, polydactyly, renal abnormalities, learning disabilities, and hypogenitalism (16). Moreover, it has been reported that TRIM32 is highly expressed in the occipital lobe of patients with Alzheimer's disease compared with that in healthy controls (17). It has been shown that TRIM32 has a ubiquitin ligase activity for actin or Piasy (small ubiquitin-like modifier ligase; ref. 18). TRIM32 ubiquitinates actin in vitro down-regulates endogenous actin in HEK293 cells and interacts directly with myosin, but not with actin (19). TRIM32 regulates UVB-induced keratinocyte apoptosis through induction of nuclear factor-B by promoting the degradation of Piasy (18). Furthermore, it has been shown that TRIM32 protein expression is elevated in a mouse skin carcinogenesis model and in human skin squamous cell carcinoma and that TRIM32 mRNA expression is elevated in human head and neck squamous cell carcinoma (20, 21). However, the role of TRIM32 in the progression of carcinogenesis has not been fully clarified.

Abl-interactor 2 (Abi2) has been identified as a protein that specifically binds to both the src homology 3 (SH3) and carboxy-terminal proline-rich sequences of Abl, which has been shown to be one of nonreceptor tyrosine kinases involved in the regulation of intercellular signals (22). Abi2 promotes Abl-mediated phosphorylation of Cdc2 and inactivation of Cdc2 kinase activity, leading to suppression of cell growth (23). Coexpression of a truncated form of Abi2 with c-Abl activates the oncogenic potential of c-Abl, suggesting that the full-length Abi2 functions as a tumor suppressor (22). Furthermore, Abi family members have been reported to affect cell motility. Abi1 promotes cell motility (24), whereas NESH (Abi3) suppresses cell motility and metastatic dissemination of malignant cells (25, 26). Deletion of the SH3 domain and carboxy-terminal proline-rich sequences in Bcr-Abl prevents Abi2-mediated degradation and inhibits cell migration, suggesting that the Abi2 negatively regulates cell motility (27).

In this study, with the aim of elucidating the molecular function of TRIM32 in carcinogenesis, we identified Abi2 as a novel TRIM32-binding protein by using yeast two-hybrid screening. TRIM32 enhanced the ubiquitination and degradation of Abi2. We also found that overexpression of TRIM32 promoted cell growth, transforming activity and cell motility. In addition, we found that TRIM32 suppressed apoptosis induced by cis-diamminedichloroplatinum (II) (cDDP) in HEp2 cell lines, originating from human laryngeal squamous cell carcinoma. Our results provide evidence for a direct role of TRIM32 in carcinogenesis, cell motility, and resistance to anticancer drugs.

	Materials and Methods

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Cell culture. HEK293T, Neuro2a, and HEp2 and its cDDP-resistant variant (HEp2/cDDP) cell lines were cultured under an atmosphere of 5% CO₂ at 37°C in DMEM (Sigma Chemical Co.) supplemented with 10% fetal bovine serum (Invitrogen). HEp2 and HEp2/cDDP cells were provided by Nippon Kayaku Co. NIH 3T3 cells were cultured under the same conditions in DMEM supplemented with 10% calf serum (CS; Camblex).

Human tumor collection. Patients with head and neck squamous cell carcinoma who gave informed consent were selected for this study. Tumor and surrounding uninvolved mucosa samples in the same patient were removed during surgery and subjected to immunoblot analysis and immunostaining with anti-TRIM32 antibody (1:1,000 dilution, mouse polyclonal, Abnova), anti-cytokeratin 1/10 (0.2 µg/mL; LH1, Santa Cruz Biotechnology), anti–cytokeratin 15 (0.2 µg/mL; LHK15, Santa Cruz), anti-basic cytokeratin (0.1 µg/mL; AE3, Santa Cruz), anti-Abi2 (0.4 µg/mL; P-20, Santa Cruz), and anti–phosphorylated histone H3 (Ser¹⁰; 5 µg/mL; rabbit polyclonal, Millipore).

Cloning of cDNAs and plasmid construction. Human TRIM32 and Abi2 cDNAs were amplified from HeLa cDNA by the PCR with BlendTaq (Takara) using the following primers: 5'-GCAATGGCTGCAGCAGCAGCTTCT-3' (TRIM32-sense), 5'-CCCCTATGGGGTGGAATATCTTCT-3' (TRIM32-antisense), 5'-GCCATGGCGGAGCTGCAGATGCTG-3' (Abi2-sense), and 5'-TGCCTACTCAGAATAATGCATGAT-3' (Abi2-antisense). The amplified fragments were subcloned into pBluescript II SK⁺ (Stratagene). FLAG-tagged, HA-tagged, or Myc-tagged TRIM32 and Abi2 cDNAs were then subcloned into pCR, pCGN, and pcDNA3 (Invitrogen) for expression in eukaryotic cells, pET30a (Novagen) for the production of His₆-tagged fusion protein, pGEX-6P1 (Amersham Bioscience) for the production of glutathione S-transferase (GST)–tagged fusion protein, and pBTM116 and pACT2 (Clontech) for a yeast two-hybrid system. Deletion mutants of TRIM32 cDNA containing amino acids 65-653, 163-653, 386-653, and 1-309 were amplified by PCR and subcloned.

Yeast two-hybrid screening. Complementary DNA encoding the full-length of human TRIM32 was fused in-frame to the nucleotide sequence for the LexA domain (BD) in the yeast two-hybrid vector pBTM116. To screen for proteins that interact with TRIM32, we transfected yeast strain L40 (Invitrogen) stably expressing the corresponding pBTM116 vector with a human HeLa cDNA library (Clontech).

Transfection, immunoprecipitation, and immunoblot analysis. HEK293T cells were transfected by the calcium phosphate method and lysed in a solution containing 50 mmol/L Tris-HCl (pH 7.4), 150 mmol/L NaCl, 1% Nonidet P-40, leupeptin (10 µg/mL), 1 mmol/L phenylmethylsulfonyl fluoride, 400 µmol/L Na₃VO₄, 400 µmol/L EDTA, 10 mmol/L NaF, and 10 mmol/L sodium PPi. The cell lysates were centrifuged at 16,000 x g for 10 min at 4°C, and the resulting supernatant was incubated with antibodies for 2 h at 4°C. Protein A or G-sepharose (Amersham Pharmacia Biotech) that had equilibrated with the same solution was added to the mixture, which was then rotated for 1 h at 4°C. The resin was separated by centrifugation, washed five times with ice-cold lysis buffer, and then boiled in SDS sample buffer. For an in vivo ubiquitination assay, the cells were lysed in a solution containing 50 mmol/L Tris-HCl (pH 7.4), 0.1% SDS, 150 mmol/L NaCl, 1% Nonidet P-40, leupeptin (10 µg/mL), 1 mmol/L phenylmethylsulfonyl fluoride, 400 µmol/L Na₃VO₄, 400 µmol/L EDTA, 10 mmol/L NaF, and 10 mmol/L sodium PPi. Immunoblot analysis was performed with the following primary antibodies: anti–c-Myc (1 µg/mL; 9E10, Covance), anti-FLAG (1 µg/mL; M5, Sigma), anti-HA (1 µg/mL; HA.11, Covance), anti-HA (1 µg/mL; Y11, Santa Cruz), anti-GST (0.1 µg/mL; B-14, Santa Cruz), anti-TRIM32 (mouse polyclonal, Abnova), anti-ubiquitin (1 µg/mL; P4D1, Santa Cruz), anti–-tubulin (1 µg/mL; TU-01, ZYMED), anti-Hsp90 (1 µg/mL; 68, Transduction Laboratories), and anti–glyceraldehyde-3-phosphate dehydrogenase (1 µg/mL; 6C5, Ambion). Immune complexes were detected with horseradish peroxidase–conjugated antibodies to mouse or rabbit IgG (1:10,000 dilution, Promega) or goat IgG (1:5,000 dilution, Santa Cruz) and an enhanced chemiluminescence system (Amersham).

Recombinant proteins. GST-tagged TRIM32 was expressed in XL-1 Blue cells and then purified by reduced glutathione–sepharose beads (Roche). His₆-FLAG-tagged Abi2 was expressed in Escherichia coli strain BL21 (DE3; Invitrogen) and then purified by using ProBond metal affinity beads (Invitrogen).

In vitro pull-down assay. GST-TRIM32 (0.25 µg) and His₆-FLAG-Abi2 (0.5 µg) were mixed in 50 mmol/L Tris-HCl (pH 7.4), 150 mmol/L NaCl, and 1% Nonidet P-40 for 1 h at 4°C. The binding mixtures were incubated with anti-GST antibody for 1 h at 4°C. Protein G-sepharose was added to the mixture, and then the mixture was rotated for 1 h at 4°C. The resin was separated by centrifugation, washed five times with buffer, and then boiled in SDS sample buffer. Immunoblot analysis was performed with anti-FLAG antibody.

Pulse-chase analysis with cycloheximide. Transiently transfected HEK293T cells were cultured with cycloheximide at the concentration of 50 µg/mL and then incubated for various times. Cell lysates were then subjected to SDS-PAGE and immunoblot analysis with an antibody to FLAG.

Retroviral infection. Retroviral expression vectors for FLAG-TRIM32 wild-type (WT), FLAG-TRIM32 deletion mutant of RING-finger domain (RING), or FLAG-Abi2 was constructed with pMX-puro. Retroviral expression vector for TRIM32(WT) or c-Src(Y527F) was constructed with pMX-hyg. Retroviral expression vectors were kindly provided by Dr. Kitamura (University of Tokyo). For retrovirus-mediated gene expression, Neuro2A and NIH 3T3 cells were infected with retroviruses produced by Plat-E packaging cells and HEp2 cells were infected with retroviruses produced by Plat-A packaging cells. Cells were then cultured in the presence of puromycin (2 µg/mL) or hygromycin B (0.2 mg/mL; Sigma).

RNA interference. The small interfering RNA (siRNA) oligonucleotide sequences specific for mouse and human TRIM32 mRNA were designed by Silencer Predesigned siRNA (Ambion) and corresponded to nucleotides 808 to 826 and 150 to 168, respectively. siRNAs were transfected by siPORT NeoFX (Ambion) into NIH 3T3, HEp2, and HEp2/cDDP cells (final concentration, 10 nmol/L). After 48 h, the resulting cell lines were checked by real-time quantitative PCR and immunoblot analysis.

Real-time quantitative PCR. Total RNA (1 µg) isolated from various cell lines using Isogen (Wako) was subjected to reverse transcription with ReverTraAce (Toyobo). The resulting cDNA was subjected to real-time quantitative PCR by TaqMan gene expression assays following the manufacturer's instructions (Applied Biosystems). The assays were performed with a mouse or human TRIM32-specific TaqMan probe and primers in an ABI-PRISM 7000 Sequence Detection System (Applied Biosystems). 18S rRNA was selected as an internal control to normalize the expression levels. Each sample was tested in triplicate.

Cell cycle analysis. NIH 3T3 cell lines were incubated in DMEM with 0.1% CS for 24 h for serum starvation. The cells released from serum starvation were harvested at indicated times and suspended in a solution containing 20 mmol/L HEPES, 160 mmol/L NaCl, 1 mmol/L EGTA, and 0.04% digitonin. The cells were incubated at 37°C for 1 h in a solution with RNase A (100 µg/mL; Novagen) and propidium iodide (20 µg/mL) and then analyzed with a FACSCalibur flow cytometer and Cell Quest software (Becton Dickinson).

Sulforhodamine B assay. Cells were seeded at a density of 2,000 per well in a 96-well plate and then fixed with 10% trichloroacetic acid at indicated times. The cells were stained with 0.4% sulforhodamine B (SRB) solution, washed using 1% acetic acid, and then solubilized with 10 mmol/L Tris base. Absorbances were measured by using a plate reader at 570 nm (28, 29).

Colony formation assay. For the colony formation assay, 1 x 10⁵ cells were plated in 60-mm dishes containing 0.4% soft agar and cultured for 2 wk. The numbers of colonies with a diameter of >0.1 mm in randomized areas (1 cm²) were counted.

Wound healing assay. A six-well plate was coated overnight with 20 µg/mL fibronectin (Asahi Techno Glass) in PBS, and then cells were seeded (3 x 10⁵ per well) in DMEM with 0.1% CS overnight. The injured line was made with a cell scraper of 1 mm in width on the confluent monolayer of cells and photographed at indicated times.

Transwell migration assay. Twelve-well polycarbonate transwell migration chambers with 8-µm pores (Corning) were coated overnight on the underside with 20 µg/mL fibronectin in PBS. The lower compartment was filled with DMEM containing 0.1% CS. Cells were cultured in DMEM with 0.1% CS for 24 h and then placed at a density of 1 x 10⁵ cells in the upper part of the transwell plate and incubated for 4 h in a serum-starved condition. The cells on the upper surface of the insert were carefully removed with cotton pads. The cells on the lower surface were fixed with 3.7% formaldehyde and stained with Hoechst 33258. The number of cells that had migrated was counted under a fluorescence microscope.

Apoptosis assay. Assessment of apoptosis was performed by measurement of sub-G₁ peak and detection of cleaved caspase-3. For sub-G₁ peak, HEp2 cells were incubated with or without cDDP (25 µmol/L) for 24 h. The cells were treated with propidium iodide and then sub-G₁ peak was analyzed with a FACSCalibur flow cytometer. For cleaved caspase-3, HEp2 cells were incubated with cDDP (25 µmol/L) for various times. Cell lysates were then subjected to immunoblot analysis with anti–caspase-3 (1:1,000 dilution; 3G2, Cell Signaling) and anti–cleaved caspase-3 (Asp¹⁷⁵; 1:1,000 dilution; 5A1, Cell Signaling) antibodies.

Statistical analysis. The unpaired Student's t test was used to determine the statistical significance of experimental data.

	Results

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Elevated expression of TRIM32 in human head and neck squamous cell carcinoma. It has been reported that TRIM32 mRNA expression was elevated in human head and neck squamous cell carcinoma. Therefore, we examined the expression level of TRIM32 protein in tumor samples that had been surgically excised. Immunoblot analysis with anti-TRIM32 antibody showed that TRIM32 protein levels were considerably elevated in 70% of tumor tissues (except for samples 5, 6, and 10) compared with the levels in normal tissues in the same patient (Fig. 1A ). To determine whether overexpression of TRIM32 antigen activity depends on the volume of epithelial components in the samples, the same cell lysates were immunoblotted with antibodies to cytokeratin 1/10 and cytokeratin 15, which have frequently been found in squamous epithelium and squamous cell carcinoma, and an antibody to basic cytokeratin. Whereas the expression levels of cytokeratin 15 were elevated in normal tissues except for sample 6, those of cytokeratin 1/10 and basic cytokeratin showed no difference between tumor and normal tissues (Fig. 1A). These results suggest that overexpression of TRIM32 in tumor tissues is independent of the abundance of epithelial components. We next performed immunohistochemical analysis using squamous cell carcinoma tissues and normal tissues of the human tongue (Fig. 1B). TRIM32 proteins were detected within the cytoplasm in tumor cells but also in normal epidermal cells near the basement membrane. We also stained the same sample with anti–phosphorylated histone H3 antibody as a mitosis marker. Both tumor cells and normal epidermal cells were stained, corresponding to the results obtained by using the anti-TRIM32 antibody. These results show that the expression of TRIM32 is elevated in human head and neck carcinoma but also in normal epidermal cells during the mitotic phase.

View larger version (111K): [in this window] [in a new window] [Download PPT slide]   Figure 1. Elevated expression of TRIM32 in human head and neck squamous cell carcinoma. A, the tissue lysates from 10 pairs of tumor (T) and normal tissues (N) were subjected to immunoblot analysis with anti-TRIM32 antibody. B, normal and tumor tissues in the same patient with tongue squamous cell carcinoma were stained with anti-TRIM32, anti-Abi2, and anti–phosphorylated specific histone H3 (Ser10) antibodies or with preimmune antibody (Control). Micrographs were obtained at 100x magnification (scale bar, 200 µm) and each black rectangle was magnified at 200x (scale bar, 100 µm).

View larger version (23K): [in this window] [in a new window] [Download PPT slide]   Figure 2. TRIM32 interacts with Abi2. A, in vivo binding assay between TRIM32 and Abi2. FLAG-TRIM32 and HA-Abi2 expression vectors were transfected into HEK293T cells. Cell lysates (WCL) were immunoprecipitated with anti-HA or anti-FLAG antibody and immunoblotted with anti-FLAG and anti-HA antibodies. B, interaction between endogenous TRIM32 and Abi2 in Neuro2a cells. Cell lysates were immunoprecipitated with anti-Abi2 antibody and then immunoblotted with anti-TRIM32 antibody. C, in vitro pull-down assay between TRIM32 and Abi2. Recombinant GST-TRIM32 and His6-FLAG-Abi2 were mixed in combination as indicated. The reaction mixtures were immunoprecipitated with anti-GST antibody and then immunoblotted with anti-FLAG antibody. D, specific interaction of the NHL domain in TRIM32 with Abi2. Schematic representation of TRIM32 deletion mutants is shown (left). Protein motifs are indicated. R, Ring-finger domain; B, B-box domain; Coil, coiled-coil domain; NHL, NHL domain. HEK293T cells were transfected with vectors for FLAG-Abi2 and either WT TRIM32 or deleted mutants tagged with the HA epitope. Cell lysates were immunoprecipitated with anti-HA antibody and then immunoblotted with anti-FLAG antibody.

View larger version (28K): [in this window] [in a new window] [Download PPT slide]   Figure 3. TRIM32 mediates ubiquitination and degradation of Abi2. A, in vivo ubiquitination assay for Abi2 by TRIM32. Expression vectors for Myc-Abi2, FLAG-TRIM32, and HA-ubiquitin were transfected into HEK293T cells, and cell lysates were immunoprecipitated with anti-Myc antibody and then anti-HA immunoblot analysis was performed to detect the ubiquitination of Abi2. B, pulse-chase analysis of Abi2 with TRIM32. HEK293T cells were transfected with expression vectors for FLAG-Abi2 and HA-TRIM32(WT), HA-TRIM32(RING), or an empty vector (Mock). Forty-eight hours after transfection, the cells were cultured in the presence of cycloheximide (50 µg/mL) for the indicated times. Cell lysates were then subjected to immunoblot analysis with anti-FLAG and anti-Hsp90 antibodies (left). Intensity of the FLAG-Abi2 bands was normalized by that of the corresponding Hsp90 bands and then expressed as a percentage of the normalized value for time 0 (right). C, down-regulation of endogenous Abi2 by TRIM32. Neuro2a cells infected with a retrovirus encoding FLAG-TRIM32(WT), FLAG-TRIM32(RING), or Mock were incubated with or without LLnL (10 µmol/L) for 4 or 8 h, and cell lysates were subjected to immunoblot analysis with anti-Abi2 antibody. The intensity of Abi2 bands was normalized by that of the corresponding -tubulin bands, and ratio of Mock at time zero was defined as 1. D, stabilization of endogenous Abi2 by RNA interference for TRIM32. The TRIM32 mRNAs or proteins derived from NIH 3T3 cells transfected with siRNA specific for mouse TRIM32 (si-TRIM32) or with nontargeting siRNA as a control (si-control) and from nontransfected cells were measured by real-time quantitative PCR or immunoblot analysis. Cell lysates were also immunoblotted with anti-Abi2 and anti–-tubulin antibodies. The intensity of Abi2 bands was normalized by that of the corresponding -tubulin bands.

View larger version (24K): [in this window] [in a new window] [Download PPT slide]   Figure 4. TRIM32 affects cell growth and cell cycle. A, acceleration of cell proliferation by TRIM32. NIH 3T3 cells infected with a retrovirus encoding FLAG-TRIM32(WT), FLAG-TRIM32(RING), or the corresponding empty vector (Mock) were seeded at 1 x 104 cells in six-well plates and harvested for determination of cell number at indicated times (left). The same experiment was performed using NIH 3T3 cells transfected with siRNA specific for mouse TRIM32 (si-TRIM32) or nontargeting siRNA as a control (si-control; right). Points, means of values from three independent experiments; bars, SD. B, TRIM32 facilitates cell cycle reentry. NIH 3T3 cells infected as above were incubated in DMEM with 0.1% CS for 24 h for serum starvation. The cells released from serum starvation were harvested at indicated times and then analyzed using a flowcytometer. C, TRIM32-mediated inhibition of suppression of cell proliferation by Abi2. NIH 3T3 cells were infected with a retrovirus encoding FLAG-Abi2 or the corresponding empty vector (Mock), and then some of the cells overexpressing FLAG-Abi2 were additionally infected with a retrovirus encoding TRIM32. The cells were counted by the same procedure as that described in A. D, colony formation assay of NIH 3T3 cell lines in soft agar. NIH 3T3 cell lines indicated in A were further infected with a retrovirus for c-Src(Y527F) and then seeded at 1 x 105 cells in 60-mm dishes containing 0.4% soft agar and cultured for 2 wk. The numbers of colonies with a diameter of >0.1 mm in randomized areas (1 cm2) were counted. Columns, means of values from three independent experiments; bars, SD. P values for the indicated comparisons were determined by Student's t test.

Furthermore, to determine whether TRIM32 affects cell transformation of overexpressed c-Src, we established NIH 3T3 cell lines stably expressing the active form of c-Src(Y529F) by retroviral infection. The resulting cell line was further infected with recombinant retroviruses encoding FLAG-tagged TRIM32(WT) or TRIM32(RING). These NIH 3T3 cell lines were then assayed for their ability to form colonies in soft agar to evaluate their ability to undergo anchorage-independent growth. The cells that had not been infected c-Src(Y529F) formed few colonies, whereas cells expressing c-Src(Y529F) formed many colonies. The combination of c-Src(Y529F) and TRIM32(WT) increased the ability of anchorage-independent growth (Fig. 4D). These findings suggest that TRIM32 functions as a positive regulator for anchorage-independent growth in collaboration with c-Src.

TRIM32 induces NIH 3T3 cell motility. Abi family proteins have been reported to mediate cell motility. Thus, we examined whether TRIM32 affects cell motility by degradation of Abi2. First, we performed a wound healing assay using several stably transfected NIH 3T3 cell lines. As shown in Fig. 4A, TRIM32 increased cell proliferation rates. Therefore, NIH 3T3 cell lines were cultured under the condition of serum starvation to arrest the cells at G₀-G₁ phase to rule out the effect of cell proliferation. TRIM32(WT) facilitated repair of cell injury more rapidly than Mock, whereas TRIM32(RING) and si-TRIM32 suppressed cell injury repair (Fig. 5A and B ). To further confirm the effect of TRIM32 on cell motility, we performed a transwell migration assay. NIH 3T3 cell lines were precultured in DMEM with 0.1% CS and then incubated in the top of the chamber for 4 h. The migration assay clarified that TRIM32(WT) increases the number of cells migrating compared with Mock but that TRIM32(RING) and si-TRIM32 do not (Fig. 5C and D). These results indicate that TRIM32 enhances NIH 3T3 cell motility and that the RING-finger domain of TRIM32 is indispensable for activation of cell motility.

View larger version (36K): [in this window] [in a new window] [Download PPT slide]   Figure 5. TRIM32 enhances NIH 3T3 cell motility. A, wound healing assay. NIH 3T3 cell lines indicated in Fig. 4A were cultured in wells coated with 20 µg/mL fibronectin in DMEM with 0.1% CS for 24 h and then an injured line was made on the confluent monolayer of cells. Cells were then incubated in serum-free medium and photographed at indicated times. Scale bar, 200 µm. B, the width of the injury line was measured at three random positions and then averaged. Points, means of values from three independent experiments; bars, SD. P values for the indicated comparisons were determined by Student's t test. C, transwell migration assay. NIH 3T3 cell lines precultured in DMEM with 0.1% CS for 24 h were seeded at 1 x 105 cells into the top of the chamber coated with 20 µg/mL fibronectin and incubated for 4 h. Cells that had migrated were fixed in formaldehyde and stained with Hoechst 33258. Scale bar, 100 µm. D, the number of cells that had migrated was counted within nine fields per insert using a fluorescence microscope. Columns, means of values from three independent experiments; bars, SD. P values for the indicated comparisons were determined by Student's t test.

View larger version (23K): [in this window] [in a new window] [Download PPT slide]   Figure 6. TRIM32 suppresses apoptosis induced by cDDP. A, effects of cDDP on cell survival of HEp2 and its cDDP-resistant variant (HEp2/cDDP). Cells were plated on 96-well plates and then incubated in the absence or presence of various concentrations of cDDP for 48 h. Cell survival was estimated using an SRB assay. Points, means of values from six independent experiments (left); bars, SD. Endogenous TRIM32 expression in HEp2 and Hep2/cDDP cells. Cell lysates were subjected to real-time quantitative PCR with a human TRIM32-specific probe and to immunoblot analysis with antibodies to TRIM32 and to -tubulin. The intensity of TRIM32 bands was normalized by that of the corresponding -tubulin bands (right). B, SRB assay. HEp2 cells infected with a retrovirus encoding FLAG-TRIM32(WT), FLAG-TRIM32(RING) or the corresponding empty vector (Mock) were plated on 96-well plates and then incubated with cDDP (5 µmol/L) for 48 h. HEp2 and HEp2/cDDP cells transfected with siRNA specific for human TRIM32 (si-TRIM32) or nontargeting siRNA as a control (si-control) were also incubated with cDDP (HEp2, 5 µmol/L; HEp2/cDDP, 20 µmol/L). Cell survival was estimated using SRB assay. Columns, means of values from six independent experiments; bars, SD. P values for the indicated comparisons were determined by Student's t test. C, measurement of sub-G1 peak. HEp2 cell lines indicated in B were incubated with cDDP (25 µmol/L) for 24 h. The cells were treated with propidium iodide, and then sub-G1 peak was analyzed with a FACSCalibur flow cytometer. Columns, means of values from three independent experiments; bars, SD. P values for the indicated comparisons were determined by Student's t test. D, detection of cleaved caspase-3. HEp2 cell lines indicated in B were incubated with cDDP (25 µmol/L) for various times. Cell lysates were then subjected to immunoblot analysis with an antibody to cleaved caspase-3.

	Discussion

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Abi2 also has been reported to mediate cell motility (27). Other Abi family proteins, including Abi1 and Abi3 (NESH), have been reported to be regulators of cell motility (24–26). Abi1 and Abi3 are localized at the edge of lamellipodial protrusions and form a complex with WAVE2. Abi1 promotes cell motility, whereas Abi3 suppresses cell motility. Abi2 has been reported to localize predominantly in the cytosol (26) and impair cell motility on the basis of results showing that a deletion mutant of Bcr-Abl lacking the ability to degrade Abi2 prevented cell migration (27). We also found that Abi2 was localized in the cytosol of HEp2 cells (Supplementary Fig. S1) and that TRIM32 enhanced cell migration, supporting the results of previous studies regarding Abi2. TRIM32 might induce cell motility via the degradation of Abi2 and mediate the invasion of tumor cells and distant metastasis. These findings may contribute new information for elucidation of the activities and possible roles in cancer of TRIM32. However, in this study, we did not determine whether the effects of TRIM32 on cell cycle, cell motility, and apoptosis directly depend on the change in activities of Abi2. Further studies are needed to clarify the functional interaction between TRIM32 and Abi2.

Moreover, our study showed that TRIM32 inhibits apoptosis induced by cDDP in HEp2 cells. Development acquired resistance to cDDP occurs commonly in patients with relapse and is a major clinical problem. The mechanism by which cancer cells become resistant to cDDP is not completely understood, although various possibilities have been suggested. For example, it is likely that cDDP is inactivated by thiol-containing molecules, such as glutathione and metallothionein, which are abundant in cells. An increasing cellular thiol content and an elevated activity of GST, which is responsible for the conjugation of cDDP to the thiol molecules, have been reported in many cDDP-resistant cell lines (32–34). As another possible mechanism, up-regulation of the ATP-binding cassette transporter family called efflux pumps, which decrease the accumulation of drugs, has been reported (35). In addition, increased DNA repair, due to an increased level of repair enzymes or DNA-binding proteins recognizing damaged DNA, has been reported in several cDDP-resistant cell lines (36, 37). Differential gene expression in cDDP-sensitive and cDDP-resistant cells has been investigated in recent studies to analyze the molecular mechanism involved in cDDP resistance (38). Our results suggest that TRIM32 contributes to the acquirement of resistance to cDDP. In conclusion, TRIM32 is a novel mediator affecting tumor growth, metastasis, and resistance to cDDP, and results of further studies on TRIM32 may be useful for establishing new chemotherapy for head and neck carcinoma.

	Disclosure of Potential Conflicts of Interest

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No potential conflicts of interest were disclosed.

	Acknowledgments

 
Grant support: Ministry of Education, Culture, Sports, Science and Technology grants 18013001 and 18390079 and Sagawa Foundation for Promotion of Cancer Research (S. Hatakeyama).

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 T. Kitamura for the plasmids and cell lines.

	Footnotes

 
Note: Supplementary data for this article are available at Cancer Research Online (http://cancerres.aacrjournals.org/).

Received 11/13/07. Revised 4/30/08. Accepted 5/14/08.

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