TRIM67 Protein Negatively Regulates Ras Activity through Degradation of 80K-H and Induces Neuritogenesis*

Background: TRIM67, which is selectively expressed in the cerebellum, is a novel member of the TRIM protein family. Results: TRIM67 interacts with PRG-1 and 80K-H, which is involved in the Ras-mediated signaling pathway. Conclusion: TRIM67 regulates Ras signaling via degradation of 80K-H, leading to neural differentiation including neuritogenesis. Significance: Analysis of TRIM67 would provide therapeutic benefits for neurodegenerative diseases. Tripartite motif (TRIM)-containing proteins, which are defined by the presence of a common domain structure composed of a RING finger, one or two B-box motifs and a coiled-coil motif, are involved in many biological processes including innate immunity, viral infection, carcinogenesis, and development. Here we show that TRIM67, which has a TRIM motif, an FN3 domain and a SPRY domain, is highly expressed in the cerebellum and that TRIM67 interacts with PRG-1 and 80K-H, which is involved in the Ras-mediated signaling pathway. Ectopic expression of TRIM67 results in degradation of endogenous 80K-H and attenuation of cell proliferation and enhances neuritogenesis in the neuroblastoma cell line N1E-115. Furthermore, morphological and biological changes caused by knockdown of 80K-H are similar to those observed by overexpression of TRIM67. These findings suggest that TRIM67 regulates Ras signaling via degradation of 80K-H, leading to neural differentiation including neuritogenesis.

The ubiquitin-mediated proteolytic pathway has an important role in the elimination of short-lived regulatory proteins (1), including those that contribute to the cell cycle, cellular signaling in response to environmental stress or extracellular ligands, morphogenesis, secretion, DNA repair, and organelle biogenesis (2). The system responsible for the attachment of ubiquitin to the target protein consists of several components that act in concert (3,4), including a ubiquitin-activating enzyme (E1), a ubiquitin-conjugating enzyme (E2) and a ubiquitin-protein isopeptide ligase (E3). E3 is thought to be the component of the ubiquitin conjugation system that is most directly responsible for substrate recognition (4). On the basis of structural similarity, E3 enzymes have been classified into three families: the HECT (homologous to E6-AP C terminus) 2 family (2,5), the RING finger-containing protein family (6 -8), and the U-box family (9 -11). The superfamily of tripartite motif-containing (TRIM) proteins is defined by the presence of a tripartite motif composed of a RING domain, one or two B-box motifs and a coiled-coil region (12,13). Many TRIM proteins are induced by type I and type II interferons (IFNs), suggesting that TRIM proteins have an important role in antiviral and anti-microbial systems (14).
It has been reported that TRIM9 is highly expressed in the cerebral cortex in mouse and human brains and that TRIM9 is decreased in damaged brains in patients who have Parkinson disease and dementia with Lewy bodies (15). TRIM9 plays an important role in the regulation of neuronal functions and participates in the pathological process of Lewy body disease (15). Overexpression of the Caenorhabditis elegans homolog of TRIM9 induces ventral axon outgrowth and ectopic branching in anterior lateral microtubule (ALM) mechanosensory neurons (16). C. elegans TRIM9 is important for axon ventral guidance in response to the attractive UNC-6/Neritin-1 signal, and Drosophila TRIM9 is required for Netrin-mediated midline attraction of sensory axons (17).
Protein kinase C substrate 80K-H (80K-H), also known as glucosidase II ␤, which encodes a soluble protein rich in glutamic and aspartic acid with putative endoplasmic reticulum (ER) retention signal at the C-terminal region (18), has been identified as a molecule downstream of fibroblast growth factor receptor (FGFR) 1 and keratinocyte growth factor receptor (19). 80K-H directly binds activated FGFR1 and forms a ternary complex with growth factor receptor-bound protein 2 (GRB2) and son of sevenless (SOS) (19). This complex formation is important in the signal pathway from FGFR1 to Ras (19 -21). 80K-H has also been identified as a molecule that interacts with the epithelial Ca 2ϩ channel, transient receptor potential cation channel V5 (TRPV5), protein kinase C and MUNC18c (22). Recently, 80K-H has been shown to interact with inositol 1,4,5trisphosphate (IP 3 ) receptors and to regulate IP 3 -induced calcium release (23). Moreover, it has been reported that 80K-H is one of the genes responsible for autosomal dominant polycystic liver disease (24,25).
Lysophosphatidic acid (LPA) is a hydrophilic lipid that acts as a ligand for intracellular signaling and induces cell proliferation, retraction, cell survival, migration, and differentiation (26 -28). Plasticity-related genes (PRGs), which are specifically expressed in the brain, are transmembrane proteins with lipid phosphate phosphatase (LPP) activity and function as receptors of LPA, resulting in regulation of least five small G-proteins (27,28). PRG-1 is an important molecule in the control of hippocampal excitability dependent on presynaptic LPA 2 receptor signaling (29). PRG-1 is likely to be a calmodulin (CaM)-interacting protein and is involved in postsynaptic functions regulated by intracellular Ca 2ϩ signaling (30). Deletion of Prg-1 in mice leads to epileptic seizures and augmentation of excitatory postsynaptic current (EPSC) but not inhibitory postsynaptic current (IPSC) (29). In utero electroporation of PRG-1 into deficient animals revealed that PRG-1 modulates excitation at the synaptic junction (29).
Based on database analysis of TRIM family proteins, we found that TRIM67, which is selectively expressed in the cerebellum, is a novel member of the TRIM protein family. The amino acid sequence of TRIM67 is similar to that of TRIM9, which has already been reported to be highly expressed in the brain. In this study, with the aim of elucidating the molecular function of TRIM67, we performed yeast two-hybrid screening using TRIM67 as bait and identified PRGs and 80K-H as TRIM67-interacting proteins. We found that TRIM67 regulates PRG-1 and 80K-H, which is involved in the activation of Ras, suggesting that TRIM67 negatively regulates Ras in cell proliferation and differentiation of neural precursor cells.
Yeast Two-hybrid Screening-Complementary DNA encoding the full length of TRIM67 or TRIM9(⌬R) was fused inframe to the nucleotide sequence for the LexA domain (Clontech Laboratories, Inc. Mountain View, CA) in the yeast two-hybrid vector pBTM116. To screen for proteins that interact with TRIM67, we transfected yeast strain L40 (Invitrogen, Carlsbad, CA) stably expressing the corresponding pBTM116 vector with a mouse brain cDNA library in pACT (Clontech) by the lithium acetate method.
Protein Stability Assay with Cycloheximide-Cells were cultured with cycloheximide (Sigma) at the concentration of 50 g/ml and then incubated for various times. Cell lysates were then subjected to SDS-PAGE and immunoblot analysis with antibodies to 80K-H, PRG-1, FLAG, and ␤-actin.
Ni-NTA Pull-down Assay-Cell lysates containing 8 M urea were used for purification of His 6 -ubiquitin-conjugated proteins by chromatography on ProBond resin (Invitrogen), and proteins were then eluted from the resin with a solution con-taining 50 mM sodium phosphate buffer (pH 8.0), 100 mM KCl, 20% glycerol, 0.2% Nonidet P-40, and 200 mM imidazole.
In Vitro Pull-down Assay-GST-TRIM67 (10 g), anti-TRIM67 antibody (10 g) and protein A-Sepharose beads (10 l) were mixed in binding buffer containing 50 mM Tris-HCl (pH 7.4), 150 mM NaCl, and 0.1% Triton X for 30 min at 4°C. The beads were then incubated with GST-80K-H (2 g) in binding buffer for 30 min at 4°C. The resin was washed five times with the buffer and then boiled in SDS sample buffer. Immunoblot analysis was performed with anti-80K-H antibody.
N1E-115 cells were lysed in a solution containing 50 mM Tris-HCl (pH 7.4), 150 mM NaCl, 1% Nonidet P-40, leupeptin (10 g/ml), 1 mM phenylmethylsulfonyl fluoride, 400 M Na 3 VO 4 , 400 M EDTA, 10 mM NaF, and 10 mM sodium pyrophosphate. The cell lysates were immunoprecipitated with anti-80K-H or anti-PRG-1 antibody and protein A-Sepharose. The resin was washed five times with the buffer and was then mixed with GST-TRIM67 (5 g) in a buffer containing 50 mM Tris-HCl (pH 7.4), 150 mM NaCl, and 0.1% Triton X for 30 min at 4°C. The resin was washed five times with the buffer and then boiled in SDS sample buffer. Immunoblot analysis was performed with anti-TRIM67 antibody.

Establishment of Stable Transfectants by Using a Retrovirus Expression System-Complementary
DNAs were subcloned into pMX-puro (kindly provided by T. Kitamura, University of Tokyo) (31). The resulting vectors were used to transfect Plat-E cells, and then recombinant retroviruses were generated (32). Forty-eight hours after transfection, culture supernatants were harvested and then used for infection into N1E-115 and HeLa cells in which mCAT-1 is stably expressed (33). The infection was carried out in the presence of polybrene at 8 g/ml (Sigma).

FIGURE 1. Localization of TRIM67 in the cerebellum and HeLa cells.
A, generation of anti-TRIM67 polyclonal antibodies. Four lots of anti-TRIM67 antibodies (anti-TRIM67-1 to -4) were established. The lysates from cells transfected with an expression vector encoding FLAG-tagged TRIM67 or FLAG-tagged TRIM9 or the lysate from the cerebellum were used for immunoblot analysis with these antibodies. ␤-actin is shown as a loading control. B, immunofluorescence analysis of TRIM67. The cells were fixed and stained with antibodies to FLAG (green), TRIM67 (red), and Hoechst33258 (blue). Anti-FLAG staining (green) showed the subcellular localization of FLAG-TRIM67 or TRIM9 expressed in HeLa cells. Staining using anti-TRIM67-1 antibody (red) showed the cytoplasmic expression of TRIM67. Scale bar, 10 m. C, tissue expression of TRIM67 in mice. The lysates from several tissues were subjected to immunoblot analysis with anti-TRIM67 antibody. ␤-Actin is shown as a loading control. D, expression of TRIM67 in mouse brain tissues. Lysates from cerebrum, cerebellum, brain stem, and spine tissues were subjected to immunoblot analysis with anti-TRIM67-1, -80K-H, and -PRG-1 antibodies. GAPDH is shown as a loading control. E, expression of TRIM67 in the human brain. Lysates from the cerebrum and cerebellum were subjected to immunoblot analysis with anti-human TRIM67, -80K-H, and PRG-1 antibodies. GAPDH is shown as a loading control.
The infected clones were expanded and selected in a medium containing puromycin (5 g/ml).
Ras Activation Assay-The amount of Ras activation was determined according to the protocol of manufacturer (Thermo Fisher Scientific, Bonn, Germany).
RNA Interference-pSUPER-retro-puro vector was purchased from OligoEngine (Seattle, WA). A short hairpin RNA (shRNA) for mouse TRIM67 or 80K-H mRNA was designed according to a previous report (34) and chemically synthesized (Invitrogen). pSUPER-retro-puro containing an shRNA for mouse TRIM67 or 80K-H sequences was constructed according to the manufacturer's protocol: shTRIM67-1, 5Ј-GAAGCTA-CGCCAGTCCACG-3Ј; shTRIM67-2, 5Ј-CAGATCTCAGA-CGCCTTG-3Ј; sh80K-H-1, 5Ј-GTGGTGACCAGCACCA-CGG-3Ј; sh80K-H-2, 5Ј-GCCATGTTCCTGAGGCCCC-3Ј. We also used a scrambled shRNA as a negative control with no significant homology to any known gene sequences in human and mouse genomes. All shRNA sequences were controlled for was expressed in HEK293T cells with or without FLAG-tagged PRG-1, followed by immunoprecipitation (IP) with anti-FLAG antibody. Immunoprecipitates were subjected to immunoblot (IB) analysis with anti-HA or FLAG antibody. C, interaction between TRIM67 and PRG-2. HA-tagged TRIM67 was expressed in HEK293T cells with or without FLAG-tagged PRG-2, followed by immunoprecipitation with anti-FLAG antibody. Immunoprecipitates were subjected to immunoblot analysis with anti-HA or FLAG antibody. D, interaction between TRIM67 lacking the RING domain (TRIM67(⌬R)) and PRG-1. HA-tagged TRIM67(⌬R) was expressed in HEK293T cells with or without FLAG-tagged PRG-1, followed by immunoprecipitation with anti-FLAG antibody. Immunoprecipitates were subjected to immunoblot analysis with anti-HA or FLAG antibody. E, interaction between TRIM67(⌬R) and PRG-2. HA-tagged TRIM67(⌬R) was expressed in HEK293T cells with or without FLAG-tagged PRG-1, followed by immunoprecipitation with anti-FLAG antibody. Immunoprecipitates were subjected to immunoblot analysis with anti-HA or FLAG antibody. F, TRIM67, TRIM9, and PRG-1 bind to 80K-H. FLAG-tagged TRIM67, FLAG-tagged TRIM9, or FLAG-tagged PRG-1 was expressed in HEK293T cells with or without HA-tagged 80K-H, followed by immunoprecipitation with anti-FLAG antibody. Immunoprecipitates were subjected to immunoblot analysis with anti-HA or FLAG antibody. G, interaction of endogenous TRIM67 with PRG-1 and 80K-H in N1E-115 cells. Cell lysates were immunoprecipitated with anti-TRIM67, anti-PRG-1, or anti-80K-H antibody and then immunoblotted with anti-TRIM67, anti-PRG-1, or anti-80K-H antibody. H, in vitro binding assay using purified recombinant TRIM67 and 80K-H proteins. Each protein was mixed in the binding buffer and rotated for 1 h. The mixture was immunoprecipitated with anti-TRIM67 and then immunoblotted with anti-TRIM67 or anti-80K-H antibody. I, interaction between recombinant TRIM67 and purified 80K-H and PRG-1 from the N1E-115 cell line. Endogenous 80K-H and PRG-1 were immunoprecipitated from N1E-115 cells using anti-80K-H or anti-PRG-1 antibody, mixed with recombinant TRIM67 and then rotated for 1 h. Immunoprecipitates were subjected to immunoblot analysis with anti-TRIM67, anti-80K-H or anti-PRG-1 antibody. their specificity by using the BLAST database. All of the above sequences were inserted into the BglII and HindIII enzyme sites of pSUPER-retro-puro vector. Approximately 50% confluent HEK293 cells in 100-mm dishes were transfected with 10 g of pSUPER-retro-puro-TRIM67, pSUPER-retro-puro-80K-H, or scrambled shRNA vector together with 10 g of amphotrophic packaging plasmid pCL10A1 using the calcium phosphate method. Forty-eight hours after transfection, culture supernatant containing retrovirus was collected, and retroviral supernatant was added to N1E-115 cells in 60-mm dishes with polybrene (8 g/ml, Sigma). Cells were cultured with puromycin (5 g/ml) for 1 week. After selection in a medium containing puromycin, the resulting cell lines were checked by immunoblot analysis with anti-TRIM67 and anti-80K-H antibodies.
Immunofluorescence Staining-HeLa cells grown on a glass cover were fixed for 10 min at room temperature with 2% formaldehyde in PBS and then incubated for 1 h at room temperature with a primary antibody in PBS containing 0.1% bovine serum albumin and 0.1% saponin. The cells were then incubated with Alexa488-labeled goat polyclonal antibody to mouse IgG or Alexa546-labeled goat polyclonal antibody to rabbit IgG (Invitrogen) at a dilution of 1:1,000. The cells were further incubated with Hoechst33258 (0.3 g/ml) in PBS for 30 s followed by extensive washing with PBS and then photographed with a CCD camera (DP71, Olympus, Japan) attached to an Olympus BX51 microscope.
Human Tissue Samples-Tissues from patients who gave informed consent under the guidelines of the Hokkaido University Hospital Ethics Committee were used for this study. All excised tissues were immediately placed in liquid nitrogen and stored at Ϫ80°C until further analysis.
Statistical Analysis-Student's t test was used to determine the statistical significance of experimental data.

Tissue Distribution and Subcellular Localization of TRIM67-
Since we found that TRIM67 seems to be selectively expressed in the brain, based on database analysis (BioGPS), we isolated mouse full-length TRIM67 cDNA. By using this cDNA, recombinant TRIM67 protein was generated to use it as an immunogen. We generated several anti-TRIM67 antibodies (TRIM67-1-4) by immunization of recombinant TRIM67 into rabbits (Fig. 1A). The amino acid sequence of TRIM67 is similar to that of TRIM9: the percent identity between TRIM67 and TRIM9 is 64.8%. Immunoblot analysis showed that four established anti-TRIM67 antibodies recognize FLAG-tagged TRIM67 but not FLAG-tagged TRIM9, indicating that these anti-TRIM67 antibodies are specific to TRIM67. In addition, immunofluorescence analysis using FLAG-tagged TRIM67-or TRIM9transfected HeLa cells showed that the staining pattern with anti-TRIM67 antibody is similar to that with anti-FLAG antibody, by which FLAG-tagged TRIM67 is stained in the cytosol or the vesicles, and that anti-TRIM67 antibody does not recognize FLAG-tagged TRIM9, which is stained in the cytosol and in the dots by anti-FLAG antibody (Fig. 1B). Immunoblot analysis using several mouse and human tissues showed that TRIM67 is highly expressed in the cerebellum (Fig. 1, C and E). Moreover, immunoblot analysis showed that TRIM67 is also highly expressed in the brainstem and spinal cord, whereas TRIM67 is weakly expressed in the cerebrum (Fig. 1, C and D).
Identification of TRIM67-binding Proteins-To identify proteins that interact with TRIM67 and TRIM9, we screened a mouse brain cDNA library with TRIM67 as a bait by the yeast two-hybrid system. We identified PRG-2 as a TRIM67-interacting protein (supplemental Fig. S1A). We further screened the mouse brain cDNA library with TRIM9(⌬R), which lacks the RING domain necessary for ubiquitin ligase activity, as a bait and isolated PRG-1 and 80K-H ( Fig. 2A, supplemental Fig.  S1, B and C). Because it has been reported that PRGs have five members, PRG-1 as another PRG member also was evaluated to examine the interaction with TRIM67. We transfected expres- sion vectors encoding HA-tagged TRIM67 and FLAG-tagged PRG-1 or FLAG-tagged PRG-2 into HEK293T cells, followed by immunoprecipitation and immunoblotting with anti-FLAG or HA antibody (Fig. 2, B and C). Immunoblot analysis showed that HA-tagged TRIM67 specifically interacts with FLAGtagged PRG-1 and FLAG-tagged PRG-2. Moreover, HA-tagged TRIM67(⌬R) specifically interacted with FLAG-tagged PRG-1 and FLAG-tagged PRG-2, suggesting that the RING domain is not required for interaction between TRIM67 and PRG-1/2 ( Fig. 2D and E). We also checked the interactions among 80K-H, PRG-1, TRIM67, and TRIM9. FLAG-tagged TRIM67, FLAG-tagged TRIM9 FLAG-tagged PRG-1 and/or HA-tagged 80K-H were transfected into HEK293T cells, and cell lysates were subjected to immunoprecipitation and immunoblotting with antibodies to FLAG or HA. Immunoblot analysis showed that 80K-H interacts with TRIM67, TRIM9, and PRG-1 (Fig.  2F). Furthermore, we verified interaction among endogenous TRIM67, PRG-1, and 80K-H by using the mouse neuroblastoma cell line N1E-115, in which endogenous TRIM67 is likely to be expressed (Fig. 2G). Immunoprecipitation analysis showed that anti-TRIM67 immunoprecipitates contained endogenous PRG-1 and 80K-H. Anti-PRG-1 and anti-80K-H  APRIL 6, 2012 • VOLUME 287 • NUMBER 15 immunoprecipitates contained enodogenous 80K-H and PRG-1, respectively. However, anti-PRG-1 and anti-80K-H immunoprecipitates did not contain endogenous TRIM67, suggesting that anti-PRG-1 and anti-80K-H antibodies recognize the binding regions between PRG-1 and TRIM67 and between 80K-H and TRIM67. Furthermore, in vitro binding assays showed direct interactions between TRIM67 and 80K-H using each purified recombinant protein (Fig. 2H). However, we could not show a direct interaction between TRIM67 and PRG-1 by an in vitro pull-down assay (data not show). We performed a pull-down assay using recombinant TRIM67 and purified 80K-H and PRG-1 prepared from N1E-115 cells (Fig. 2I). Immunoblot analysis showed that recombinant TRIM67 interacts with 80K-H and PRG-1 purified from N1E-115 cells. These findings indicate that TRIM67 directly interacts with 80K-H and suggest that TRIM67 interacts with PRG-1 via an unknown modification or unknown adaptor molecule.

TRIM67 Regulates Neuritogenesis
TRIM67 Promotes Ubiquitination and Degradation of 80K-H but Not Those of PRG-1-We first established N1E-115 cell lines stably expressing FLAG-tagged TRIM67 and FLAGtagged TRIM67(⌬R) (Fig. 3A). A protein stability assay with cycloheximide using these cell lines was performed to examine the effect of stability of 80K-H by TRIM67. Ectopic expression of TRIM67 resulted in rapid degradation of endogenous 80K-H compared with mock, whereas TRIM67(⌬R) delayed the degradation of 80K-H, suggesting that the RING domain of TRIM67 is required for acceleration of degradation of 80K-H (Fig. 3A). Interestingly, the stability of PRG-1 was increased by TRIM67, suggesting that TRIM67 stabilizes PRG-1 possibly via their interaction (Fig. 3B). Since TRIM67 promoted degradation of 80K-H, we performed an in vivo ubiquitination assay of 80K-H in the presence of TRIM67. The in vivo ubiquitination assay showed that TRIM67 overexpression enhances ubiquitination of 80K-H, suggesting that TRIM67 promotes ubiquitination of 80K-H and then contributes to the proteasomal degradation of 80K-H (Fig. 3C).
Neural Differentiation of N1E-115 by TRIM67-Because it has been reported that serum starvation results in neurite outgrowth and differentiation of N1E-115 cells (35) and that PRG-1 mediates neurite outgrowth (27,36), we analyzed the physiological roles of TRIM67 using N1E-115 cells. To clarify the functional effect of TRIM67 on differentiation of N1E-115 cells, we investigated morphological change of N1E-115 cells under a serum starvation condition (Fig. 4A). In the presence of serum, TRIM67 overexpression induced a flattened shape and extended neurites compared with the mock cell line (Fig. 4,  A and B). After serum starvation for 24 h, TRIM67 or TRIM67(⌬R) overexpression increased the number of neuritebearing cells, but the effect of TRIM67(⌬R) was weaker than that of TRIM67, suggesting that the RING domain is partially required for neuritogenesis (Fig. 4, A and B). Furthermore, TRIM67 or TRIM67(⌬R) overexpression attenuated cell proliferation, followed by neural differentiation (Fig. 4C).
Because it has been reported that 80K-H and PRG-1 regulate Ras activity (28,37), we examined the biological function of TRIM67 in a Ras activation. We pulled-down activated Ras with the Ras-binding domain of Raf using stable N1E-115 cell line overexpressing FLAG-TRIM67 and investigated the amount of the GTP-bound active form Ras. The Ras activation assays showed that Ras is inactivated in N1E-115 cells by overexpression of TRIM67, suggesting that TRIM67 causes delayed cell proliferation and enhanced neuritogenesis because of inactivation of Ras via inhibition of 80K-H (Fig. 4, D and E).
Up-regulation of Ras Activity by Knockdown of TRIM67-To examine the physiological role of TRIM67, we knocked down endogenous TRIM67 in N1E-115 cells by using two independent targeting sequences (Fig. 5A). Knockdown of TRIM67 caused up-regulation of 80K-H, indicating that TRIM67 may be an E3 ubiquitin ligase for 80K-H (Fig. 5A). Furthermore, knockdown of TRIM67 in N1E-115 cells slightly but significantly reduced the number of neurite-bearing cells in the presence of TRIM67 Regulates Neuritogenesis serum (Fig. 5, B and C). Furthermore, knockdown of TRIM67 caused acceleration of cell growth (Fig. 5D). To examine the effect of knockdown of TRIM67 on Ras activation, we compared the amount of active Ras in TRIM67 knocked-down cell lines compared with that in mock cells. Activation of Ras was observed in TRIM67 knocked-down cell lines but not in mock cells (Fig. 5E). These findings suggest that TRIM67 negatively regulates Ras activation.
Differentiation of N1E-115 Cells by Knockdown of 80K-H-To clarify the physiological relationship between TRIM67 and 80K-H, we also established two independent 80K-H knockeddown N1E-115 cell lines (Fig. 6A). Using these cell lines, we counted the number of neurite-bearing cells in the presence of serum. Knockdown of 80K-H caused an increase in the number of neurite-bearing cells compared with mock cells in the presence of serum (Fig. 6, B and C). Furthermore, knockdown of 80K-H attenuated cell proliferation (Fig. 6D). Given that the physiological phenotype of 80K-H knockdown is similar to that of TRIM67 overexpression and that TRIM67 physically interacts with 80K-H, TRIM67 may function as a negative regulator for 80K-H, resulting in Ras inhibition via degradation of 80K-H followed by growth arrest and neuritogenesis in neural precursor cells.

DISCUSSION
In this study, we identified PRG-1 and 80K-H as TRIM67interacting proteins. We showed that TRIM67 functioned as a putative E3 ubiquitin ligase for 80K-H and that ectopic expression of TRIM67 induced neurite outgrowth and suppressed growth of N1E-115 cells. Moreover, ectopic expression of TRIM67 down-regulated Ras activity probably via degradation of 80K-H. In contrast, knockdown of TRIM67 attenuated neurite outgrowth in N1E-115 cells and up-regulated Ras activity. The regulation of cell proliferation has been shown to be tightly linked to differentiation in normal cells including neurons and also tumor cells with deregulated proliferation (38,39). These findings suggest that TRIM67 attenuates cell proliferation and induces morphological changes like neuronal differentiation.
FGF stimulation induces tyrosine phosphorylation of 80K-H, which binds activated FGFR directly and forms a ternary complex with GRB2-SOS, leading to a connection from FGFR to the Ras signal (19,20,37). Our studies showed that morphological and biological effects by knockdown of 80K-H were similar to the changes induced by overexpression of TRIM67. These findings indicate that overexpression of TRIM67 in N1E-115 cells may downregulate activation of Ras via degradation of 80K-H. Furthermore, it has been reported that TRIM9 has an E3 ubiquitin ligase activity and affects the localization of downstream effectors by ubiquitinating Rac guanine nucleotide exchange factor (GEF) (15,17). Since TRIM67 is structurally similar to TRIM9, TRIM67 may also function as an E3 ubiquitin ligase for 80K-H as a regulator for Ras,. It has been reported that Purkinje cells from IP 3 R-deficient mice show abnormal dendritic outgrowth (40). 80K-H interacts with inositol 1,4,5-trisphosphate receptors (IP 3 R), regulates IP 3 -induced calcium release and consequently contributes to neuronal functions (23). Taken together, the results indicate that IP 3 R may be functionally inhibited by TRIM67 through degradation of 80K-H, resulting in regulation of neuronal differentiation.
PRG-1 is highly expressed in the forebrain and in the cerebellar cortex (30). It has been reported that overexpression of PRG-1 induces neurite outgrowth in PC12 cells (36) and that PRG-1 is up-regulated during periods of axonal outgrowth and attenuates LPA-induced axon collapse (27). PRG-1 deficiency results in pathological network synchronization due to a pathological increase of excitatory synaptic transmission (29). In this study, we showed that overexpression of TRIM67 may stabilize endogenous PRG-1, indicating that neurite outgrowth by overexpression of TRIM67 is due to stabilization of PRG-1.
Considering that overexpression of TRIM67 in N1E-115 cells causes stabilization of PRG-1, TRIM67 may function as a positive regulator for PRG-1. Because deletion of prg-1 in mice leads to epileptic seizures, TRIM67 and TRIM9 may be associated with the etiology of epilepsy (29). Hence, it would be interesting to clarify the molecular mechanism of TRIM67 in epilepsy.
In conclusion, TRIM67 interacts with PRG-1 and 80K-H and affects neurite elongation in neuronal precursor cells. However, it is unclear whether interaction of TRIM67 with PRG-1 and 80K-H contributes to neuronal development. Genetic approaches using transgenic or knock-out mice will be necessary to clarify the relationship between TRIM67 and neuritogenesis. Further functional analysis of TRIM67 at the molecular level would provide therapeutic benefits not only for suppression in axonal injury but also for neurodegenerative diseases.