The Identification of Histidine 712 as a Critical Residue for Constitutive TRPV5 Internalization*

The epithelial Ca2+ channel TRPV5 constitutes the apical entry gate for Ca2+ transport in renal epithelial cells. Ablation of the trpv5 gene in mice leads to a reduced Ca2+ reabsorption. TRPV5 is tightly regulated by various calciotropic hormones, associated proteins, and other factors, which mainly affect channel activity via the C terminus. To further identify the role of the C terminus in TRPV5 regulation, we expressed channels harboring C-terminal deletions and studied channel activity by measuring intracellular Ca2+ concentration ([Ca2+]i) using fura-2 analysis. Removal of amino acid His712 elevated the [Ca2+]i, indicating enlarged TRPV5 activity. In addition, substitution of the positively charged His712 for a negative (H712D) or neutral (H712N) amino acid also stimulated TRPV5 activity. This critical role of His712 was confirmed by patch clamp analysis, which demonstrates increased Na+ and Ca2+ currents for TRPV5-H712D. Cell surface biotinylation studies revealed enhanced plasma membrane expression of TRPV5-H712D as compared with wild-type (WT) TRPV5. This elevated plasma membrane presence also was observed with the Ca2+-impermeable TRPV5-H712D and TRPV5-WT pore mutants, demonstrating that the elevation is not due to the increased [Ca2+]i. Finally, using an internalization assay, we demonstrated a delayed cell surface retrieval for TRPV5-H712D, likely causing the increase in plasma membrane expression. Together, these results demonstrate that His712 plays an essential role in plasma membrane regulation of TRPV5 via a constitutive endocytotic mechanism.

The epithelial Ca 2؉ channel TRPV5 constitutes the apical entry gate for Ca 2؉ transport in renal epithelial cells. Ablation of the trpv5 gene in mice leads to a reduced Ca 2؉ reabsorption. TRPV5 is tightly regulated by various calciotropic hormones, associated proteins, and other factors, which mainly affect channel activity via the C terminus. To further identify the role of the C terminus in TRPV5 regulation, we expressed channels harboring C-terminal deletions and studied channel activity by measuring intracellular Ca 2؉ concentration ([Ca 2؉ ] i ) using fura-2 analysis. Removal of amino acid His 712 elevated the [Ca 2؉ ] i , indicating enlarged TRPV5 activity. In addition, substitution of the positively charged His 712 for a negative (H712D) or neutral (H712N) amino acid also stimulated TRPV5 activity. This critical role of His 712 was confirmed by patch clamp analysis, which demonstrates increased Na ؉ and Ca 2؉ currents for TRPV5-H712D. Cell surface biotinylation studies revealed enhanced plasma membrane expression of TRPV5-H712D as compared with wild-type (WT) TRPV5. This elevated plasma membrane presence also was observed with the Ca 2؉ -impermeable TRPV5-H712D and TRPV5-WT pore mutants, demonstrating that the elevation is not due to the increased [Ca 2؉ ] i . Finally, using an internalization assay, we demonstrated a delayed cell surface retrieval for TRPV5-H712D, likely causing the increase in plasma membrane expression. Together, these results demonstrate that His 712 plays an essential role in plasma membrane regulation of TRPV5 via a constitutive endocytotic mechanism.
Calcium (Ca 2ϩ ) plays a critical role in many cellular and physiological processes in the human body. Ca 2ϩ homeostasis is maintained via the interplay between intestinal absorption, storage in bone, and renal excretion. Excretion of Ca 2ϩ by the kidney is regulated through the reabsorption of Ca 2ϩ from the glomerular filtrate. This takes place in the proximal tubule and thick ascending limb of Henle via a passive paracellular pathway driven by the Na ϩ gradient, whereas in the distal part of the nephron, Ca 2ϩ is reabsorbed actively in a trans-cellular man-ner. The epithelial Ca 2ϩ channel TRPV5 (transient receptor potential vanilloid 5) forms the apical entry gate for transepithelial Ca 2ϩ reabsorption (1,2). When Ca 2ϩ enters the cell, it is bound by calbindin-D 28k and released at the basolateral site where Ca 2ϩ is extruded into the bloodstream by the Na ϩ /Ca 2ϩ exchanger (NCX1) and the plasma membrane Ca 2ϩ -ATPase (PMCA1b). The apical influx of Ca 2ϩ is the rate-limiting step in transepithelial Ca 2ϩ transport. This becomes evident in the tight control of TRPV5 protein expression, channel trafficking, and gating at the plasma membrane by various hormones, associated proteins, and other factors (3,4). Moreover, disruption of the trpv5 gene in mice resulted in profound hypercalciuria due to diminished active Ca 2ϩ reabsorption (5).
TRPV5 belongs to the superfamily of TRP channels, which share the mutual composition of six transmembrane domains and permeability to cations (6). A functional TRPV5 channel consists of four identical subunits, forming a single central pore located between transmembrane domains five and six (7). Within the mammalian TRP family, TRPV5 and its closest homologue TRPV6 are the most Ca 2ϩ -selective channels (6). Furthermore, TRPV5 is constitutively open at low [Ca 2ϩ ] i and is characterized by an inward rectifying ion current-voltage (I-V) profile (8). The membrane-spanning region is flanked by large intracellular N and C termini (9). The N terminus contains several ankyrin repeats, which have been implicated in channel assembly (10,11). However, the molecular function of these ankyrin repeats remains controversial (12,13).
Although the function of the TRPV5 N terminus still is largely unresolved, the C terminus plays a central role in TRPV5 channel regulation. Various molecular processes, including protonation, phosphorylation, and protein-protein interactions, affect TRPV5 activity by modulating the C terminus. First, Huang and co-workers (14) found that binding of protons to lysine 607 induced a conformational change of the channel pore, mainly resulting in a reduced channel open probability. Second, the protein kinase A phosphorylation site Thr 709 of TRPV5 was identified recently as a target for parathyroid hormone. Protein kinase A-dependent phosphorylation of Thr 709 rapidly increases TRPV5 channel open probability and thereby enhances Ca 2ϩ influx (15). Third, the C-terminal PKC phosphorylation site Ser 654 appears essential for tissue kallikrein-mediated plasma membrane accumulation of TRPV5 (16). Fourth, the C-terminal VATTV sequence is required for S100A10-TRPV5 interaction. Alanine substitution of the first threonine, T599A, prevents S100A10 binding to TRPV5, leading to the subplasma membrane localization of TRPV5 and thus a nonfunctional channel (17). Fifth, Rab11a targets TRPV5 toward the plasma membrane via C-terminal interaction (18).
Finally, the TRPV5 C terminus has been shown convincingly to be involved in Ca 2ϩ -dependent inactivation. Two Ca 2ϩsensing stretches were identified in the TRPV5 C terminus, one between residues 650 and 653 and the other in the last 30 residues (19). Deleting both stretches resulted in a channel that does not inactivate in the presence of a concentration of 1 M intracellular Ca 2ϩ (19). In addition, removing only the last 30 residues significantly diminished the Ca 2ϩ -dependent inactivation of TRPV5 (19). To explore the exact role of this highly regulated part of the C terminus, we developed a series of TRPV5 C-terminal deletion mutants. The role of these mutants in TRPV5 channel regulation were tested with a combination of live-cell imaging, patch clamp analysis, and various biochemical approaches.

Construction of Mammalian Expression Vectors-
The bicistronic expression vector pCINeo/IRES-eGFP was used to coexpress rabbit TRPV5 containing an N-terminally fused HAtag and enhanced green fluorescent protein (eGFP). C-terminal truncations and mutations of TRPV5 were produced by PCR and site-directed mutagenesis (Stratagene), according to the manufacturer's protocol, after which all plasmids were sequence-verified.
[Ca 2ϩ ] i Measurement using Fura-2/AM-HEK293 cells were seeded on fibronectin-coated coverslips (inner diameter, 25 mm) and transfected with the appropriate pCINeo/IRES-eGFP vector. After 24 h, cells were loaded with 3 M fura-2/AM and 0.01% (v/v) Pluronic F-129 (both from Molecular Probes) in DMEM medium at 37°C for 20 min. After loading, cells were washed twice with PBS and allowed to equilibrate at 37°C for another 10 min in 132.0 mM NaCl, 4.2 mM KCl, 1.4 mM CaCl 2 , 1.0 mM MgCl 2 , 5.5 mM D-glucose, 10 mM HEPES/Tris, pH 7.4. For Ca 2ϩ -free conditions, a similar buffer composition was used, in which Ca 2ϩ was substituted with 2 mM EGTA.
After fura-2 loading, cells were placed in an incubation chamber and attached to the stage of an inverted microscope (Axiovert 200M, Carl Zeiss, Jena, Germany). Changes in extracellular [Ca 2ϩ ] ([Ca 2ϩ ] e ) were facilitated using a perfusion system and resulting changes in [Ca 2ϩ ] i were monitored with fura-2 and were excited at 340 and 380 nm using a monochromator (Polychrome IV, TILL Photonics, Gräfelfing, Germany). Fluorescence emission light was directed by a 415DCLP dichroic mirror (Omega Optical, Inc., Brattleboro, VT) through a 510WB40 emission filter (Omega Optical, Inc.) onto a Cool-SNAP HQ monochrome CCD-camera (Roper Scientific, Vianen, the Netherlands). The integration time of the CCDcamera was set at 200 ms with a sampling interval of 3 s. All hardware was controlled with Metafluor (version 6.0) software (Universal Imaging Corp., Downingtown, PA).
Quantitative image analysis was performed with Metamorph (version 6.0; Molecular Devices Corp., Sunnyvale, CA). For each wavelength, the mean fluorescence intensity was monitored in an intracellular region and, for purpose of background correction, an extracellular region of identical size. After background correction, the fluorescence emission ratio of 340 and 380 nm excitation was calculated to determine the [Ca 2ϩ ] i . All measurements were performed at room temperature.
Cell Surface Biotinylation and Internalization Assay-HEK293 cells were transfected with different TRPV5 con- structs in pCINeo/IRES-eGFP using PEI. After 2 days, cell surface proteins were biotinylated for 30 min at 4°C using sulfo-NHS-LC-LC-biotin or sulfo-NHS-SS-biotin (0.5 mg/ml; Pierce) as described previously (21). In short, cells were kept at 4°C or incubated for 30 min at 37°C to allow endocytosis from the plasma membrane. TRPV5 internalization was measured by treating cells with fresh 100 mM 2-mercaptoethanesulfonic acid sodium salt (mesna) for three times for 20 min at 4°C. After treatment with 120 mM iodoacetic acid to quench mesna, cells were lysed in 150 mM NaCl, 5 mM EGTA, 50 mM Tris-HCl, pH 7.5, Triton X-100 1% (v/v), and protease inhibitors at 4°C and centrifuged at 14,000 ϫ g for 10 min. Finally, biotinylated proteins in the supernatant were precipitated using neutravidin-coupled beads (Pierce) and analyzed by immunoblotting using anti-HA antibodies.
Statistical Analysis-Numerical results were visualized using Origin Pro 7.5 (OriginLab Corp., Northampton, MA) and presented as the mean Ϯ S.E. Statistical differences were determined using a one-way ANOVA followed by Bonferroni. p values Ͻ0.05 were considered significant.

Removal of the Very End of TRPV5 C Terminus Elevates [Ca 2ϩ ] i -To study TRPV5 function in intact cells, we monitored [Ca 2ϩ
] i using fura-2. To this extent, HEK293 cells were seeded on fibronectin-coated coverslips and transiently transfected with TRPV5 in pCINeo/IRES-eGFP or the empty vector. After 24 h, cells were loaded with fura-2/AM, equilibrated for 10 min, and placed on the stage of an inverted microscope. Cells expressing eGFP were selected and monitored for changes in [Ca 2ϩ ] i in response to variation of ([Ca 2ϩ ] e , which was facilitated by superfusion. Expression of the TRPV5 channel resulted in an elevated [Ca 2ϩ ] i compared with mock-transfected cells (Fig. 1, A and C). When medium containing 1.4 mM Ca 2ϩ was exchanged for Ca 2ϩ -free medium (no Ca 2ϩ , 2 mM EGTA), the [Ca 2ϩ ] i in TRPV5-expressing cells dropped to levels similar to mocktransfected cells. Exchanging the Ca 2ϩ -free medium again for the 1.4 mM Ca 2ϩ solution induced an overshoot; a rapid increase of [Ca 2ϩ ] i to a maximal level followed by a gradual decrease to basal levels. No significant changes in [Ca 2ϩ ] i were observed in mock-transfected cells (Fig. 1, A and C).
Next, HEK293 cells were transfected with a TRPV5 mutant lacking a part of the C terminus (TRPV5-698X). Previously, a similar mutant displayed a blunted response to Ca 2ϩ -induced channel inactivation as measured by patch clamp analysis (19). Fura-2 analysis of TRPV5-698X-expressing HEK293 cells revealed an elevated basal [Ca 2ϩ ] i compared with TRPV5-WT. TRPV5-698X responded only partially to EGTA treatment (Fig. 1, B and C). Replacing the EGTA medium with Ca 2ϩ medium restored [Ca 2ϩ ] i to basal levels after a small overshoot (Fig. 1, B and C).
Functional Analysis of C-terminal Deletion Mutants Reveals Residue His 712 -To pinpoint the region responsible for the elevated [Ca 2ϩ ] i observed in cells expressing TRPV5-698X, shorter deletions within the TRPV5 C terminus were made ( Fig.  2A). Deletions up to residue His 712 did not affect resting [Ca 2ϩ ] i as shown in Fig. 2B. However, deletion of His 712 (TRPV5-712X) resulted in a significant increased basal [Ca 2ϩ ] i , although not as high as the 698X mutation (Fig. 2B). Remarkably, fura-2 peak levels (maximal [Ca 2ϩ ] i ) of TRPV-712X were identical to TRPV5-698X as indicated by Fig. 2C. Maximal [Ca 2ϩ ] i of the shorter deletion mutants were identical to TRPV5-WT. All C-terminal deletions were correctly expressed as judged by immunoblotting (Fig. 2D).
As His 712 is positively charged, we examined whether this charge is responsible for the observed effect on [Ca 2ϩ ] i of TRPV5-712X. Mutation of His 712 into a negatively charged aspartic acid (TRPV5-H712D) or a neutral asparagine (TRPV5-H712N) enlarged basal [Ca 2ϩ ] i to a similar extent as TRPV5-712X (Fig. 3A). In contrast, replacement of His 712 with the positively charged arginine (TRPV5-H712R) did not modulate the intracellular Ca 2ϩ levels (Fig. 3A). Analysis of the peak fura-2 levels of these mutants resulted in an identical [Ca 2ϩ ] i pattern as observed at basal conditions (Fig. 3B). Immunoblotting did not demonstrate large variations in protein expression (Fig. 3C). Interestingly, His 712 is highly conserved among different mammalian species (Fig. 3D).
Critical role of His 712 Is Independent of Protein Kinase A-dependent Phosphorylation-Residue His 712 is located very close to a conserved protein kinase A-dependent phosphorylation site 706 RRNT*LGH 712 . Upon phosphorylation of Thr 709 , the channel open probability increases, resulting in an elevated TRPV5-mediated Ca 2ϩ influx (15). To investigate whether deletion or mutation of His 712 affects TRPV5 activation by protein kinase A-dependent phosphorylation, we used the cAMPelevating agent forskolin and studied its effect on TRPV5 activity using fura-2 analysis. First, to confirm the specificity of the forskolin response, we implemented a phosphorylationdeficient mutant (T709A) and one mimicking a constitutively phosphorylated state (T709D). Forskolin increased [Ca 2ϩ ] i of cells expressing TRPV5-WT, whereas mock-expressing cells were not affected (Fig. 4, A and C). Fura-2 ratio of cells expressing T709A and T709D was not altered upon forskolin stimulation (Fig. 4, B and C). Notably, basal [Ca 2ϩ ] i of the T709D mutant was elevated significantly in comparison with TRPV5-WT and TRPV5-T709A (Fig. 4C) and similar to [Ca 2ϩ ] i of the TRPV5-H712D mutant.
Next, the forskolin response on TRPV5-712X and TRPV5-H712D was examined. Although basal [Ca 2ϩ ] i of TRPV5-712X and TRPV5-H712D was already elevated compared with TRPV5-WT, forskolin treatment resulted in a dramatic increase in [Ca 2ϩ ] i (Fig. 4, D and E). In addition, we developed a double mutant by introducing the T709D mutation into TRPV5-H712D. This double mutant exhibited a similar [Ca 2ϩ ] i as TRPV5-H712D after forskolin stimulation (Fig. 4, F and G). Furthermore, neither the double mutant nor TRPV5-698X responded to forskolin (Fig. 4, F and G).
TRPV5-H712D Elevates Channel Plasma Membrane Abundance-To gain more insight into the molecular features of the TRPV5-H712D mutant, we compared the fura-2 recording traces of TRPV5-H712D and TRPV5-T709D in response to the Ca 2ϩ and Ca 2ϩ -free medium. Both mutants displayed a similarly increased basal [Ca 2ϩ ] i , which fully decreased in Ca 2ϩ -free medium (EGTA treatment) (Fig. 5A). Interestingly, the maximal [Ca 2ϩ ] i of TRPV5-H712D was significantly elevated in comparison with TRPV5-T709D (Fig. 5,  A and B).
To investigate whether [Ca 2ϩ ] i plays a role in the elevated activity observed for TRPV5-H712D, the whole cell patch clamp technique was implemented, and Ca 2ϩ and Na ϩ currents of TRPV5-WT and TRPV5-H712D were evaluated. Application of a hyperpolarizing voltage step to Ϫ100 mV from a holding potential of ϩ70 mV showed an increased Ca 2ϩ peak current in H712D-expressing cells compared with TRPV5-WT cells (Fig. 5, C and  5D). Na ϩ current measurements in nominally divalent-free solution (20 M EDTA) demonstrated that TRPV5-H712D still exhibited an enlarged macroscopic current (Fig. 5, E and F). The strong inward rectification, which is characteristic for the TRPV5 channel, should also be noted (Fig. 5E) (20).
To identify the mechanism underlying the amplified currents of TRPV5-H712D, plasma membrane expression was assessed. A cell surface biotinylation was conducted on HEK293 cells transfected with either TRPV5-WT or TRPV5-H712D. Ten minutes before biotinylation, cells were stimulated with forskolin. Subsequently, cells were lysed, and biotinylated proteins were precipitated with neutravidin-agarose beads, and TRPV5 expression was studied using immunoblotting. Plasma membrane presence of the H712D mutant was elevated clearly in comparison with TRPV5-WT (Fig. 6, A and B). Forskolin stimulation did not affect plasma membrane presence of either protein. Importantly, expression of TRPV5-WT and TRPV5-H712D in whole cell lysates was similar. As a control for H712D, the positively charged arginine 707 was replaced by glutamic acid (R707E). Plasma membrane expression of R707E was not different from TRPV5-WT (supplemental Fig. 1).
In 2008, de Graaf et al. (21) reported that [Ca 2ϩ ] i increases TRPV5 recycling toward the plasma membrane. To verify that the increased plasma membrane expression of TRPV5-H712D was due directly to the H712D mutation and not secondary to an elevated [Ca 2ϩ ] i , the pore mutation D542A was introduced. This mutation impedes Ca 2ϩ selectivity, whereas Na ϩ still permeates the channel. Plasma membrane expression of TRPV5-D542A-H712D was increased (Fig. 6, C and D), whereas [Ca 2ϩ ] i was not different from TRPV5-D542A or mock (data not shown).
Plasma Membrane Retrieval of TRPV5-H712D Is Delayed-To elucidate how TRPV5-H712D plasma membrane abundance is elevated, an internalization assay was performed using HEK293 cells expressing TRPV5-WT or TRPV5-H712D. In short, cell surface proteins were probed with sulfo-NHS-SS- biotin, and cells were incubated for 30 min at 37°C to allow internalization of biotinylated proteins. Finally, cells were treated with the membrane-impermeant mesna, removing all biotin bound to remaining cell surface proteins. In agreement with the previous figure, TRPV5-H712D plasma membrane presence was increased (Fig. 7A, no mesna). Mesna treatment removed ϳ80% of the biotin attached to TRPV5 proteins in both TRPV5-WT and TRPV5-H712D (Fig. 7, A and B, no  chase). A 30-min incubation at 37°C increased the mesna-resistant fraction of TRPV5-WT by ϳ40% (Fig. 7, A and B, 30-min chase). In contrast, only an additional ϳ20% of biotinylated TRPV5-H712D was resistant to mesna. Importantly, expres-sion of TRPV5-WT and TRPV5-H712D in total cell lysates was similar (Fig. 7C). This experiment demonstrates that retrieval rate of TRPV5-H712D channels from the cell surface is significantly slower than TRPV5-WT.

DISCUSSION
In this study, we identified the C-terminally located His 712 as a critical residue for constitutive TRPV5 internalization. This conclusion is based on the following observations. First, functional analysis of C-terminal deletion mutants demonstrated the importance of residue His 712 in the regulation of TRPV5 activity. Second, substitution of the positively charged His 712 for a neutral or negative residue increased TRPV5 activity. Third, the effects observed for H712D were independent of protein kinase A-mediated phosphorylation of the nearby residue T709. Fourth, cell surface biotinylation revealed an increased abundance of TRPV5-H712D channels at the plasma membrane. Fifth, TRPV5-H712D exhibited a delayed internalization from the cell surface, likely causing the increased plasma membrane presence.
We employed fura-2 analysis to investigate TRPV5 function. Fura-2 is a ratiometric dye and readout of [Ca 2ϩ ] i is, therefore, independent of the dye concentration, illumination intensity, and optical path length. ] i , is likely a specific TRPV5 characteristic, as it was not observed in cells expressing the heterologous channel TRPV6 (data not shown). This phenomenon might be due to the relatively slow Ca 2ϩ -induced inactivation of TRPV5 compared with TRPV6 (22).
Using fura-2 analysis, a critical role for the positive charge of His 712 in regulating TRPV5 activity was identified, as deletion or substitution resulted in enhanced channel activity. Residue His 712 is in close proximity to the conserved protein kinase A phosphorylation site Thr 709 regulating TRPV5 open probability by the calciotropic hormone parathyroid hormone (15). As substitution of both Thr 709 and His 712 by a negatively charged residue elevated basal [Ca 2ϩ ] i to a similar extent, we investigated whether both mutants concealed a similar activation mechanism. Nevertheless, protein kinase A-mediated stimulation by forskolin was not compromised in TRPV5-H712D, suggesting independent pathways for the elevated TRPV5 activity. This was confirmed by fura-2 analysis of the maximal [Ca 2ϩ ] i , which revealed that the overshoot of [Ca 2ϩ ] i of TRPV5-H712D was increased significantly in comparison with T709D. This implies that the elevated basal activity of both mutants is caused by two distinct molecular mechanisms. Indeed, the T709D mutant leads to an increase in channel open probability (15), whereas cell surface biotinylation studies demonstrated an increased plasma membrane abundance of TRPV5-H712D. Thus, an enlarged maximal [Ca 2ϩ ] i , as detected by fura-2 analysis, implies an elevation in TRPV5 plasma membrane expression. Moreover, replacing the positively charged Arg 707 by glutamic acid (R707E) did not affect the cell surface expression of TRPV5, demonstrating the specific role for His 712 in TRPV5 plasma membrane trafficking.
Interestingly, introduction of the D542A mutation, which prevents Ca 2ϩ influx, further increased plasma membrane expression of TRPV5-H712D (supplemental Fig. 2). This indicates that a high [Ca 2ϩ ] i , as present in cells expressing TRPV5-H712D, prevents full plasma membrane accumulation of this mutant. This is in contrast with observations in neuronal cells, where intracellular Ca 2ϩ elevations induce synaptic vesicle fusion and reduce endocytosis, resulting in an elevated plasma membrane presence of synaptic ion channels (23,24).
Finally, an internalization assay was implemented to study the role for residue His 712 in TRPV5 channel retrieval. Pilot experiments did not reveal any internalization of TRPV5-H712D after a 5-min incubation at 37°C, FIGURE 5. TRPV5-H712D exhibits an enlarged Ca 2؉ and Na ؉ current. A, representative trace of fura-2 ratio in HEK293 cells transiently transfected with TRPV5-T709D and TRPV5-H712D. B, fura-2 levels in arbitrary units (a.u.) at basal conditions (t ϭ 0) and peak level (max) upon administration of 1.4 mM Ca 2ϩ . Average data of TRPV5-T709D (n ϭ 19) and TRPV5-H712D (n ϭ 22) as depicted in white and black bars, respectively. The asterisk denotes a significant difference (p Ͻ 0.05) from indicated condition. C, inward Ca 2ϩ currents measured with 10 mM extracellular Ca 2ϩ during a 3-s step to Ϫ100 mV from a holding potential of ϩ70 mV in HEK293 cells expressing either TRPV5-WT or TRPV5-H712D. D, average peak current density during a voltage step to Ϫ100 mV in 10 mM Ca 2ϩ . Cells expressing TRPV5-H712D displayed significantly increased Ca 2ϩ peak currents. *, p Ͻ 0.05 compared with TRPV5-WT. E, I-V relationship measured from 450-ms voltage ramps in nominally divalentfree solution. F, average current densities at Ϫ80 mV in nominally divalent-free solution. Cells expressing H712D displayed significantly increased Na ϩ currents at Ϫ80 mV. *, p Ͻ 0.05 compared with TRPV5-WT. which was detected for TRPV5-WT. Analysis after 30 min of incubation at 37°C demonstrated a significant delayed channel retrieval for the H712D mutant, which ultimately results in an increased plasma membrane abundance. Recent investigations shed light on the process of TRPV5 retrieval from the plasma membrane. In 2007, de Graaf et al. (21) found that constitutive TRPV5 internalization is clathrin-dependent. Cha et al. (25) demonstrated the involvement of caveolae in TRPV5 endocytosis. PKC stimulation via parathyroid hormone or 1oleoyl-2-acetyl-sn-glycerol activated TRPV5 via an enhanced plasma membrane expression, which was absent in cells treated with caveolin-1 siRNA or caveolin-1-negative cells (25). Using the dominant-negative dynamin mutant K44A, both studies revealed a crucial role for dynamin in TRPV5 endocytosis. In addition, TRPV5 plasma membrane expression is regulated by various physiological stimuli including the ␤-glucuronidase klotho, tissue kallikrein, and extracellular pH (16,26,27). In this study, we identified the first residue within TRPV5 essential for constitutive internalization. It is not yet clear whether physiological stimuli can modify internalization via His 712 ; however, future research should unravel such a mechanism.
The critical role for His 712 also became apparent by its conservation among different mammalian species. In general, classical internalization signals (28 -30) are composed of several residues, none of them resembling the amino acids surrounding His 712 . Removal of residues after His 712 did not increase TRPV5 activity. Therefore, the contribution of the highly conserved residues upstream of His 712 (Leu 710 and Gly 711 ) in TRPV5 internalization remains to be investigated in the future. Altogether, this study demonstrated an essential role for residue His 712 in TRPV5 plasma membrane trafficking. FIGURE 7. Internalization assay demonstrates a delayed retrieval of TRPV5-H712D. A, biotinylated TRPV5-WT or TRPV5-H712D channels after treatment with mesna. NB, no biotin control. B, quantification of the biotinylated fraction of multiple experiments (n ϭ 4) corrected for protein input as shown as percentage of no mesna conditions. C, total cell lysate of TRPV5-WT or TRPV5-H712D transfected HEK293 cells as referred to as protein input.