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RESEARCH ARTICLE |
1 Zentrum für Molekulare Neurobiologie, Universität Hamburg, Martinistraße 52, 20246 Hamburg, Germany
2 Institut für Physiologie, Universität Hamburg, Martinistraße 52, 20246 Hamburg, Germany
3 Institute for Molecular and Cellular Regulation, Gunma University, Maebashi 371-8512, Japan
* These authors contributed equally to this work
Author for correspondence (e-mail: schaller{at}zmnh.uni-hamburg.de)
Accepted July 13, 2001
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SUMMARY |
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Key words: Head-activator signaling, Ion-channel trafficking, Receptor-mediated calcium entry, GRC, VRL-1, PI3-K, CaMK, TRP-like channel
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INTRODUCTION |
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TopSUMMARYINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONREFERENCES |
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Growth factors stimulate cell proliferation by inducing Ca2+ entry into cells. Recently, a new Ca2+-permeable channel was cloned from mouse spleen that controls proliferation of cells responsive to insulin-like growth factor-1 (IGF-1), platelet-derived growth factor (PDGF) and serum. It was named growth-factor-regulated channel (GRC) by Kanzaki et al. (Kanzaki et al., 1999). Rat and human homologues were described by Caterina et al. (Caterina et al., 1999) and called vanilloid-receptor like (VRL-1) because of their similarity to the capsaicin receptor VR1. Both GRC and VRL-1 have almost identical biophysical and pharmacological properties and represent orthologues of the same channel. GRC belongs to the transient receptor potential (TRP) channel family members of which allow Ca2+ entry into cells at hyperpolarized membrane potentials (Clapham et al., 2001; Harteneck et al., 2000). GRC contains six transmembrane domains, a pore loop, a cytoplasmic N-terminus with three ankyrin repeats, and a cytoplasmic C-terminus. CHO cells transfected with GRC reacted to IGF-1, PDGF and serum by translocation of this channel from an intracellular pool to the plasma membrane and by an increase in intracellular Ca2+ concentration. The effect of IGF-1 and PDGF on GRC translocation was indirect and required activation of the phosphatidylinositol 3-kinase (PI3-K) (Kanzaki et al., 1999). Capsaicin did not affect GRC channel properties, but high noxious heat activated the channel (Caterina et al., 1999). So far it is unclear which endogenous ligands or second messengers are responsible for GRC activation. Expression of VRL-1/GRC in sensory neurons of dorsal-root ganglia, but also in other organs, such as spleen and lung, hint at multiple functions (Caterina et al., 1999).
Here, we show that HA-responsive cells contain GRC, that the channel translocates to the cell surface after HA application, and that Ca2+ influx through this channel is triggered by HA. HA does not bind directly to GRC, but requires the presence of a signaling receptor and respective second messengers. We propose a model how the signaling cascade induced by HA may lead to the activation of GRC as a Ca2+-permeable channel and how its trafficking from intracellular stores to the plasma membrane is regulated.
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MATERIALS AND METHODS |
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COS-7 and CHO cells were transfected by electroporation with 10 µg pcDNA3 into which nothing (mock), mouse GRC, mouse GRC-FLAG or human SorLA cDNAs were cloned. For electrical recordings, cells were microinjected with 50 ng/µl GRC-pcDNA3 and 5 ng/µl EGFP-N1-pcDNA3, the latter to facilitate detection of cells with successful expression.
PCR analysis of GRC in NT2, BON and NH15-CA2 cells
Two protein motifs conserved in GRC and VR1 (Caterina et al., 1997) were chosen to design oligonucleotides for PCR amplification, namely the sequence LLQ(DE)KWD, located five amino acids in front of the first transmembrane domain, and FKFTIGMG at the end of the pore loop to yield 5'-TTITT(GT)CAGGA(GT)AAGTGGGAT-3' as sense and 5'CCCATICC(GT)ATIGTGAA(CT)TT(AG)AA-3' as antisense primers. As templates we used cDNA from BON and NH15-CA2 cells and a commercial cDNA library from uninduced NT2 cells (Stratagene). The PCR profile was 94°C 30 seconds, 45°C 30 seconds, 72°C 45 seconds for 30 cycles, followed by re-PCR under the same conditions.
Immunostaining and confocal analysis of GRC translocation
NH15-CA2 and BON cells and transfected CHO and COS-7 cells were plated on chamber slides in serum-containing medium for 24 hours. Analysis was performed after subsequent growth in defined medium for 24 hours. HA was monomerized prior to use (Bodenmüller et al., 1986). Signal transduction was inhibited by pretreating cells for 20 minutes with 200 ng/ml pertussis toxin (Sigma), 10 µM SK&F 96365 (Biomol), 10 µM KN93 (Calbiochem), 10 µM roscovitin (Calbiochem), or 100 nM wortmannin (Calbiochem), before HA was added. To demonstrate immunoreactivity on the plasma membrane, living cells were treated with the primary antisera diluted in defined medium for 20 minutes at 37°C. After washing with PBS, cells were fixed with 4% paraformaldehyde in 7% acetic acid and 7% glycerol for 30 minutes at 21°C. To show translocation, cells were first fixed for 5 minutes in ice-cold 1% acetic acid in ethanol, before the primary antisera were added (Kanzaki et al., 1999). The GRC antiserum (Kanzaki et al., 1999) was diluted 1:2000, the FLAG antibody (FLAG M2; Sigma) 1:440 and the SorLA antiserum against the fibronectin domain 1:2000 (Hampe et al., 2000). For confocal analysis cy2- or cy3-labeled secondary antisera were used, the transfection efficiency was controlled with alkaline phosphatase-conjugated secondary antibodies.
Membrane preparation, solubilization and HA crosslinking
Cells were harvested by treatment with 2 mM EDTA in PBS for 10 minutes, collected by centrifugation, and ultrasonicated in a Tris-HCl (pH 7.4) buffer containing 2 mM EDTA and a protease-inhibitor cocktail (complete; Roche Molecular Biochemicals). After centrifugation at 100,000 g, the membrane pellets were either used for western blotting or solubilized with 1% Nonidet P-40 in 50 mM Tris-HCl (pH 7.4) and 150 mM NaCl by incubation for 30 minutes at 4°C with occasional syringe pipetting. The 100,000 g supernatant was diluted tenfold in buffer without detergent, and FLAG-tagged GRC was immunoprecipitated with anti-FLAG agarose (Sigma) overnight at 4°C with overhead tumbling. Non-bound material was removed by washing three times with Tris-buffered saline. The various fractions were mixed with sample buffer without heating and subjected to 12% polyacrylamide gel electrophoresis. After semi-dry blotting immunoreactivity was visualized by enhanced chemiluminiscence (Pierce).
To crosslink HA to cell surface proteins, cells were incubated for 10-20 minutes at 37°C with the 125I-labeled HA bipeptide (Hampe et al., 1996), washed twice with PBS, and treated with 0.1% 1-ethyl-3-(3-dimethylamino-propyl)carbodiimide-HCl (EDC; Pierce) and 0.1% N-hydroxysulfo-succinimide (sulfo-NHS; Pierce) in PBS for 20 minutes at 37°C.
Electrophysiology
Membrane currents were recorded in the whole-cell configuration (Hamill et al., 1981) or the perforated-patch configuration with nystatin (Horn and Marty, 1988) of the patch-clamp technique. An EPC9 patch-clamp amplifier was used in conjunction with the PULSE stimulation and data acquisition software (HEKA Elektronik). The patch electrodes were made from 1.5 mm diameter borosilicate glass capillaries with resistances of 2.5-4 M
when filled with intracellular solution. Data were low-pass filtered at 3 kHz and compensated for both fast and slow capacity transients. Series resistance was compensated by 75-90%. Current traces are shown without correction for leakage, taking into account that GRC shows a substantial inward current. All experiments were performed at room temperature (22-25°C).
The pipette solution contained 140 mM KCl, 2 mM MgCl2, 1 mM CaCl2, 2.5 mM EGTA, 10 mM Hepes and had a calculated free Ca2+ concentration of 66 nM. The pH was adjusted to 7.3 with KOH. The standard external solutions contained 130 mM NaCl, 2 mM MgCl2, 2 mM CaCl2, 5 mM KCl, 10 mM Hepes, and 10 mM glucose. The NaCl, CsCl and CaCl2 solutions contained 150 mM NaCl or CsCl or 100 mM CaCl2, 10 mM Hepes, 10 mM glucose, buffered to pH 7.3 with NaOH, CsOH or Ca(OH)2. Nystatin was dissolved in DMSO. Its final concentration in the standard pipette solution was 0.2 mg/ml. All chemicals for electrophysiology were purchased from Sigma.
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RESULTS |
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nor Gß/
subunits were detectable in the FLAG-GRC immunoprecipitate.
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subunit of G proteins. To assay whether SorLA is the HA receptor which triggers GRC translocation, we cotransfected CHO cells with GRC and SorLA. As in CHO cells transfected with GRC alone, HA was unable to induce GRC translocation or GRC currents (data not shown). This indicates that CHO cells miss an important component of the HA signaling cascade. |
DISCUSSION |
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TopSUMMARYINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONREFERENCES |
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We found that HA-responsive cells contain GRC and react to HA stimulation with a translocation of GRC to the cell surface. GRC could be visualized on the surface of living cells without HA stimulation, but its density increased considerably after HA application. Maximal translocation was observed in NH15-CA2 cells 30 minutes after HA treatment and returned to control levels after 60 minutes. A similar time course was observed for HA induced inward currents, which showed biophysical and pharmacological properties agreeing with those reported previously for GRC/VRL-1 by other workers (Caterina et al., 1997; Kanzaki et al., 1999). We interpret this to mean that some GRCs are always present at the outer cell membrane, that they may be responsible for the immediate stimulation of receptor-mediated Ca2+ entry, but that the sustained Ca2+ influx requires recruitment or shuttling of GRC from intracellular stores to the cell surface.
The closest relative of GRC in the TRP family is the vanilloid receptor VR-1, for which capsaicin and amandamide or other endogeneous lipids serve as ligands (Caterina et al., 1997; Hwang et al., 2000; Jung et al., 1999). These ligands are supposed to activate channel opening by directly binding to VR-1. One possible scenario for HA signaling to GRC could therefore be direct binding. To test this hypothesis we transfected COS-7 and CHO cells with GRC and measured translocation and Ca2+ influx. Whereas HA was able to trigger a response in COS-7 cells, no effect was obtained in CHO cells, although both reacted with serum. In line with this we found that radioactively labeled HA could bind to COS-7, but not to CHO cells, and that cell proliferation could be stimulated with HA in non-transfected COS-7, but not in CHO cells (data not shown). Binding of HA and internalization was speeded up in the presence of GRC, indicating that the presence of GRC enhances HA’s action. Crosslinking of HA to COS-7 cells and subsequent pull-down of FLAG-tagged GRC with FLAG agarose confirmed the notion that HA does not bind directly to GRC.
HA-stimulated translocation of GRC to the cell surface and HA-induced currents were inhibited by SK&F 96365, a specific blocker of receptor-mediated, store-independent Ca2+ entry specific for TRP-like channels (Bennett et al., 2001). SK&F 96365 prevents HA triggered mitosis and cell proliferation (Kayser et al., 1998; Ulrich et al., 1996), and it inhibits the effects of other growth factors on stimulating proliferation of astrocytoma, neuroblastoma and blood cells (Chung et al., 1994; Lee et al., 1993). SK&F 96365 leads to an arrest of cells at the G2/mitosis transition (Nordström et al., 1992). This suggests that the GRC is involved in the control of cell proliferation, mediating HA’s action at this cell-cycle checkpoint.
In the presence of pertussis toxin, the effect of HA on stimulating mitosis and cell proliferation is inhibited (Ulrich et al., 1996). Likewise, pretreatment of GRC-transfected cells with pertussis toxin inhibited HA-induced translocation of GRC to the cell surface and HA-induced currents, indicating that HA signaling for mitosis and GRC translocation and channel activation are mediated by a receptor that is coupled to an inhibitory G protein. No co-immunprecipitation of GRC with G-protein subunits was found, implying indirect activation over other second messengers. SorLA, a single transmembrane receptor that binds HA, contains motifs typical for coupling to inhibitory G proteins (Franke et al., 1997). Cotransfection of CHO cells with GRC and SorLA did not result in conferring responsiveness to HA, indicating that an additional component is missing in CHO cells. Therefore, we postulate that HA together with SorLA binds most likely to a member of the G protein-coupled receptor family, which transmits the signal over an inhibitory G protein to GRC. HA-induced translocation of GRC was blockable by inhibitors of two kinases, namely by KN-93, an inhibitor of the Ca2+/calmodulin-dependent kinases and by wortmannin, a blocker of the PI3-kinase. No effect was found with roscovitin, which blocks the cyclin-dependent kinase CDK1. A model of how these different components may interact is depicted in Fig. 10. After binding its ligand the HA-receptor complex activates a pertussis-toxin-sensitive G protein, which probably interacts via PI3-K with GRC at the cell surface to induce Ca2+ entry. The increase in Ca2+ concentration activates CaMK, which alone or together with PI3-K triggers translocation of more GRC channels to the cell surface thus leading to a prolonged Ca2+ influx.
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ACKNOWLEDGMENTS |
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; GRC, 
). (C) Activation of GRC by HA was reduced after application of 10 µM ruthenium red (RR) in an external CsCl solution. Membrane currents were recorded with a 250 ms voltage ramp command from -100 mV to 60 mV from a holding potential of -60 mV. (D) HA-activated GRC was Ca2+ permeable, if the measurement was performed in an external CaCl2 solution, and the currents were blockable by RR. (E) The membrane current of a cell expressing GRC, but not of a mock-injected COS-7 cell, increased after HA application as measured in the perforated-patch configuration using standard external NaCl solution. Membrane currents activated by HA in cells expressing GRC were blocked by application of 1 mM La3+ or 10 µM RR. Dashed lines denote zero current, arrows indicate the time of HA or blocker application (F,G). In CHO cells heterologously expressed GRC was not activated by HA (F), but by serum (G). Membrane currents were elicited as described in (C). In an external CaCl2 solution a CHO cell pretreated with HA for 20 minutes did not exhibit increased membrane currents (F). Pretreatment with 10% fetal calf serum activated GRC-mediated membrane currents, which could be reduced by 10 µM RR (G).
