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AT₁ receptor-mediated accumulation of extracellular angiotensin II in proximal tubule cells: role of cytoskeleton microtubules and tyrosine phosphatases

¹Laboratory of Receptor and Signal Transduction, Division of Hypertension and Vascular Research, Henry Ford Hospital, Detroit; ²Department of Physiology, Tulane University Health Sciences Center, New Orleans, Louisiana; and ³Department of Physiology, Wayne State University School of Medicine, Detroit, Michigan

Submitted 14 October 2005 ; accepted in final form 9 February 2006

	ABSTRACT

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Long-term angiotensin II (ANG II) administration is associated with increased ANG II accumulation in the kidney, but intrarenal compartment(s) involved in this response remains to be determined. We tested the hypothesis that 1) extracellular ANG II is taken up by proximal tubule cells (PTCs) through AT₁ receptor-mediated endocytosis, 2) this process is regulated by cytoskeleton microtubule- and tyrosine phosphatase-dependent mechanisms, and 3) AT₁ receptor-mediated endocytosis of ANG II has a functional relevance by modulating intracellular cAMP signaling. In cultured PTCs, [¹²⁵I]Tyr-labeled ANG II and fluorescein labeled-ANG II were internalized in a time-dependent manner and colocalized with the endosome marker Alexa Fluor 594-transferrin. Endocytosis of extracellular ANG II was inhibited by the AT₁ receptor blocker losartan (16.5 ± 4.6%, P < 0.01 vs. ANG II, 78.3 ± 6.2%) and by the tyrosine phosphatase inhibitor phenylarsine oxide (PAO; 30.0 ± 3.5%, P < 0.05 vs. ANG II). Intracellular ANG II levels were increased by 58% (basal, 229.8 ± 11.4 vs. ANG II, 361.3 ± 11.8 pg ANG II/mg protein, P < 0.01), and the responses were blocked by losartan (P < 0.01), the cytoskeleton microtubule inhibitor colchicine (P < 0.05), and PAO (P < 0.01), whereas depletion of clathrin-coated pits with hyperosmotic sucrose had no effect (356.1 ± 25.5 pg ANG II/mg protein, not significant). ANG II accumulation was associated with significant inhibition of both basal (control, 15.5 ± 2.8 vs. ANG II, 9.1 ± 2.4 pmol/mg protein, P < 0.05) and forskolin-stimulated cAMP signaling (forskolin, 68.7 ± 8.6 vs. forskolin + ANG II, 42.8 ± 13.8 pmol/mg protein, P < 0.01). These effects were blocked by losartan and PAO. We conclude that extracellular ANG II is internalized in PTCs through AT₁ receptor-mediated endocytosis and that internalized ANG II may play a functional role in proximal tubule cells by inhibiting intracellular cAMP signaling.

kidney; receptor-mediated endocytosis

Our group (42) recently demonstrated that increased intrarenal uptake of ANG II occurred primarily in renal cortical endosomes of ANG II-infused rats and was prevented by the AT₁ receptor blocker candesartan. However, pharmacological blockers cannot distinguish between AT₁ receptor subtypes, because there is 95% genomic homology between AT_1A and AT_1B receptors (7). Most of AT₁ receptor-mediated agonist endocytosis involves AT_1A receptors, whereas the role of AT_1B receptors remains unclear (7). To understand the role of AT₁ receptor-mediated endocytosis in renal epithelial cells, opossum kidney (OK) epithelial cells and human embryonic kidney 293 cells (HEK-293) were transfected with AT_1A receptors (16, 34), but these cells do not express major components of the renin-angiotensin system (RAS; including endogenous AT_1A receptors), and therefore their physiological relevance remains uncertain. Recent evidence suggests that AT₁ receptor-mediated endocytosis of extracellular ANG II is important not just for trafficking ANG II to the lysosomes for degradation and recycling of the receptors back to the membranes but also for full expression of the biological actions of ANG II in various cells (16, 29, 30, 34). For example, endocytosis of the ANG II-AT₁ receptor complex is accompanied by increased phospholipase C- or phospholipase A₂-mediated sodium flux and decreased cAMP production in renal epithelial cells (4, 29, 30, 34). These studies suggest that AT_1A receptor-mediated endocytosis plays an important role in regulating PTC transport.

In the present study, we hypothesized that 1) extracellular ANG II is taken up by PTCs through AT₁ receptor-mediated endocytosis; 2) receptor-mediated ANG II endocytosis contributes to increased intracellular accumulation of ANG II in PTCs; 3) blockade of receptor-mediated endocytosis by inhibitors of cell membrane cytoskeleton microtubules or tyrosine phosphatases prevents accumulation of ANG II in PTCs; and 4) AT₁ receptor-mediated ANG II endocytosis plays a physiological role by regulating intracellular cAMP signaling. Using cultured rabbit PTCs derived from the S1 segment of proximal convoluted tubules, which express major components of the RAS (including AT₁ and AT₂ receptors), we demonstrated that AT₁ receptor-mediated endocytosis of extracellular ANG II contributes to intracellular accumulation of ANG II in PTCs in vitro and plays an important role in the regulation of proximal tubule transport by modulating intracellular cAMP signaling.

	MATERIALS AND METHODS

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Materials. Cultured PTCs were obtained from American Type Culture Collection (vEPT; ATCC). These cells were initially derived from the S1 segment of rabbit kidney proximal convoluted tubules and have been shown to express electrolyte transporters as well as major components of the RAS, including angiotensinogen, renin, angiotensin-converting enzyme (ACE), and ANG II receptors (26, 27). Dulbecco's modified Eagle's medium, nutrient mixture, Ham's F-12 (DMEM/F-12), trypsin, heat-inactivated fetal bovine serum (FBS), and the antibiotics penicillin and streptomycin were purchased from ATCC. Human Val⁵-ANG II, the radioligand [¹²⁵I]Tyr-ANG II, and ANG II enzyme immunoassay kits were obtained from Biochem/Peninsula Laboratories. cAMP enzyme immunoassay kits were purchased from R&D Systems. The AT₁ receptor antagonist losartan was a gift from Merck Pharmaceuticals, and the AT₂ receptor antagonist PD-123319 was donated by Pfizer. AT₁ receptor small-inteference RNA (siRNA) and rabbit polyclonal AT₁ receptor antibody targeting the NH₂-terminal extracellular domain of the human AT₁ receptor (N-10), scrambled siRNA, and transfection reagents were purchased from Santa Cruz Biotechnology. Western blot supplies were obtained from Amersham. Colchicine and phenylarsine oxide (PAO) were obtained from Calbiochem.

Cell culture. Unless specified otherwise, PTCs (passages 8- 12) were subcultured in six-well plates in complete DMEM/F-12 growth medium supplemented with 50 nM hydrocortisone, 5% heat-inactivated FBS, 100 U/ml penicillin, and 100 µg/ml streptomycin (26, 27, 43). After reaching 80% confluence, they were starved in serum-free medium for 24 h before the experiment (26, 27, 43).

Expression of AT₁ and AT₂ receptors. To determine the proportion of AT₁ or AT₂ receptors in PTCs, we used [¹²⁵I]Tyr-ANG II binding assays as described previously (15, 39, 40). Briefly, the cells were incubated with [¹²⁵I]Tyr-ANG II (100 pmol) for 60 min at 37°C. Total ANG II receptor binding was calculated as the binding in the absence of unlabeled ANG II or its receptor subtype-selective antagonist in the incubation. Nonspecific binding was determined as the binding in the presence of 10 µM unlabeled ANG II. AT₁ receptor binding was determined in the presence of 10 µM unlabeled AT₂ receptor blocker PD-123319, whereas AT₂ receptor binding was calculated as the binding in the presence of 10 µM unlabeled AT₁ blocker losartan. To determine ANG II receptor binding affinity constant (K_d) and maximum binding capacity (B_max), we produced saturation binding curves and Scatchard plot by incubating PTCs with increasing concentrations of [¹²⁵I]Tyr-ANG II (0–10 nM) alone or with 100 pmol of [¹²⁵I]Tyr-ANG II in the presence of increasing concentrations of unlabeled ANG II or losartan (0–10 µM). K_d and B_max were calculated using GraphPad Prism 4.0.

To confirm that rabbit PTCs express AT₁ receptor protein, we divided subconfluent (60%) cells into three groups (n = 6). The first group was treated with serum-free medium as a control. The second group was transfected with an AT₁ receptor-specific 20- to 25-nucleotide siRNA (AT₁R siRNA; Santa Cruz) (37). The third group was transfected with a negative, non-AT₁ receptor-targeting, scrambled siRNA (Santa Cruz). After transfection, cells were washed twice with ice-cold phosphate-buffered saline (PBS) and lysed with a modified RIPA buffer (50 mM Tris·HCl, 1% NP-40, 0.25% Na-deoxycholate, 150 mM NaCl, 1 mM EDTA, 1 mM PMSF, 1 µg/ml each of aprotinin, leupeptin, and pepstatin, 1 mM Na₃VO₄, and 1 mM NaF, pH 7.4). Proteins were extracted, electrophoretically separated on 8–16% Tris-glycine gels, and transferred to Millipore Immobilon-P membranes. The membranes were incubated for 3 h at room temperature with a rabbit polyclonal antibody against the human AT₁ receptor (N-10, 1:200; Santa Cruz) or a rabbit anti-AT_1A receptor polyclonal antibody against the cytosolic domain of the AT_1A receptor (CLSTKMSTLSYRPSDNM; 1:200) as described (11, 17, 42, 43). Western blot signals were detected using enhanced chemiluminescence (Amersham) and analyzed using a microcomputer imaging device with a digital camera (MCID, Imaging Research, Ontario, Canada).

AT₁ receptor-mediated endocytosis of extracellular ANG II. To determine whether AT₁ receptors are internalized by PTCs when exposed to extracellular ANG II, the cells were incubated with 100 pmol [¹²⁵I]Tyr-ANG II for 2, 5, 10, 15, or 30 min at 37°C alone or in the presence of the AT₁ receptor blocker losartan (10 µM) or the specific tyrosine phosphatase inhibitor PAO (1 µM), both known to inhibit AT_1A receptor endocytosis (9, 12, 30). At each time point, incubations were stopped by washing the cells twice with ice-cold PBS to remove free radioligands from the medium. Acid-sensitive (noninternalized) and -insensitive radioactivity (internalized) were separated by washing the cells twice with 5 mM ice-cold acetic acid buffer in 150 mM NaCl, pH 2.5. Radioactivity was counted and the percentage of internalized or noninternalized receptors analyzed (2, 12, 34).

Effects of AT₁ and AT₂ receptor blockade on intracellular accumulation of ANG II. To determine the role(s) of AT₁ receptor-mediated ANG II endocytosis, PTCs were treated with vehicle (serum-free medium), ANG II (Val⁵-ANG II; 1 nM), ANG II plus losartan (10 µM), or ANG II plus PD-123319 (10 µM) for 60 min at 37°C. After treatment, the medium was removed and the cells washed twice with ice-cold PBS and then twice with ice-cold acid buffer (5 mM acetic acid, 150 mM NaCl, pH 2.5) to remove any cell membrane-bound ANG II (2, 12, 16, 34). ANG II was extracted from PTCs in a buffer containing 20 mM Tris·HCl, 10 mM EDTA, 5 mM EGTA, 5 mM mercaptoethanol, 50 g/ml PMSF, 1 µg/ml aprotinin, and 1 µg/ml pepstatin A and measured using a sensitive and specific ANG II enzyme immunoassay kit (Biochem/Peninsula).

Effects of inhibitors of clathrin-coated pits, cytoskeleton microtubules, and tyrosine phosphatase on intracellular ANG II accumulation. To determine the role(s) of clathrin-coated pits, cytoskeleton microtubules, or tyrosine phosphatases in AT₁ receptor-mediated ANG II endocytosis in PTCs, the cells were treated with serum-free medium alone, ANG II (1 nM), ANG II plus 400 mM sucrose, which depletes clathrin-coated pits (2, 9, 10), ANG II plus the cytoskeleton microtubule inhibitor colchicine (1 µM) (3, 8, 29), or ANG II plus the tyrosine phosphatase inhibitor PAO (1 µM) to block AT₁ receptor-mediated endocytosis (9, 12, 30). PAO is an established tyrosine phosphatase inhibitor that has been widely used for studying G protein-coupled receptor (GPCR) endocytosis (9, 12, 30, 33, 36). After treatment, the cells were washed and ANG II was extracted as described above.

Effects of AT₁ receptor-mediated endocytosis of extracellular ANG II on intracellular cAMP production. Cyclic AMP is one of the most important signaling molecules involved in the regulation of sodium and fluid transport by ANG II in proximal tubules (14, 22, 27, 34). ANG II is thought to activate mainly basolateral AT₁ receptors, which are coupled to adenylyl cyclase via G_i proteins, to inhibit formation of cAMP; however, it was recently reported that after endocytosis, ANG II may directly activate G_i protein-coupled basolateral AT₁ receptors (34). To determine whether AT₁ receptor-mediated ANG II endocytosis can affect intracellular cAMP signaling, we followed three experimental protocols. First, subconfluent PTCs in six-well plates were treated for 15, 30, or 60 min with serum-free medium only or ANG II (1 nM) alone to determine the time-dependent responses of cAMP production to ANG II (n = 6 each). Second, based on the time-dependent responses of cAMP to ANG II (peaked at 30 min), PTCs were pretreated with the AT₁ receptor blocker losartan (10 µM) or the tyrosine phosphatase inhibitor PAO (1 µM) before exposure to ANG II for 30 min (n = 6 each). Cells treated with losartan or PAO alone also were used as controls. Third, PTCs were treated for 30 min with 1) the adenylyl cyclase activator forskolin alone (10 µM), which stimulates cAMP production, 2) forskolin plus ANG II (ANG II + forskolin), 3) ANG II plus forskolin and the AT₁ receptor blocker losartan (10 µM), 4) ANG II plus forskolin and the AT₂ receptor blocker PD-123319 (10 µM), or 5) ANG II plus forskolin and the endocytotic inhibitor PAO (1 µM) (n = 6 each). The phosphodiesterase inhibitor 3-isobutyl-1-methylxanthine (IBMX; 1 mM) was added to all samples to prevent degradation of cAMP (29, 33). After treatment, the culture medium was removed and the cells were washed and lysed with 0.1 N HCl. The lysates were centrifuged at 1000 g, and the supernatant was collected for cAMP measurements with the use of a sensitive cAMP ELISA kit (R&D).

Statistical analysis. Results are expressed as means ± SE. Unless otherwise specified, 6–12 samples from two separate experiments were collected for each treatment and assayed in duplicate for measurements of intracellular ANG II levels. For Western blot data, at least six samples from two separate experiments were performed, with each treatment assayed in duplicate. For binding data, two separate experiments were performed, with each time point determined in duplicate. Comparisons between two treatments were made using Student's unpaired t-test. Comparisons between more than two treatments were made with one-way analysis of variance, followed by a Newman-Keuls test for multiple comparisons. P < 0.05 was considered significant.

	RESULTS

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
Expression of AT₁ receptors in rabbit proximal tubule cells. As shown in Fig. 1A, radioreceptor binding assays using [¹²⁵I]Tyr-ANG II showed that PTCs express a single class of ANG II receptor binding. Scatchard analysis suggests that these cells bound [¹²⁵I]Tyr-ANG II with an apparent K_d of 6.8 ± 2.1 nM, and the B_max averaged 1,012 ± 28 fmol/mg protein. The AT₁ receptor predominates in these cells because losartan (10 µM), a competitive AT₁ receptor blocker, displaced over 90% of total ANG II receptor binding, whereas the AT₂ receptor-selective blocker PD-123319 (10 µM) inhibited <10% of binding. Next, we used two approaches to confirm that PTCs express AT₁ receptors. First, with the use of a rabbit anti-AT₁ receptor polyclonal antibody against the NH₂-terminal extracellular domain of the human AT₁ receptor (11, 17, 42), Western blot detected a single protein band of 42 kDa (Fig. 1B). The AT₁ receptor protein we detected is consistent with the AT₁ receptor reportedly expressed in the rat kidney (15). In previous studies, pretreatment of samples with an AT₁ receptor-selective antigen blocking peptide (Santa Cruz) before running the Western blot confirmed the specificity of the AT₁ receptor protein (15, 43). Second, AT₁ receptor protein expression was significantly knocked down by 80% after transfection of PTCs with an AT₁-selective siRNA, whereas a scrambled, non-AT₁-selective siRNA had little effect (Fig. 1B). When the same membranes were stripped and reprobed with an anti--actin antibody, equal protein loading was confirmed (Fig. 1A, bottom band). Thus the PTCs we used express AT₁ receptor protein corresponding to human AT₁ receptors.

View larger version (16K): [in this window] [in a new window]   Fig. 1. Expression of AT1 receptors (equivalent to human AT1 or rodent AT1A) in cultured rabbit proximal tubule cells (PTCs). A: [125I]Tyr-ANG II receptor binding showing binding competition by the unlabeled ANG II, AT1 receptor blocker losartan or the AT2 receptor blocker PD-123319 (10–11 to 10–4 M) and Scatchard analysis of maximum binding capacity (Bmax) and the apparent Kd. B: ANG II receptor protein expression was significantly inhibited by a specific AT1 receptor small-interference RNA (AT1R siRNA), whereas a scrambled siRNA had no effect. **P < 0.01 vs. control.

View larger version (12K): [in this window] [in a new window]   Fig. 2. Time-dependent endocytosis of [125I]Tyr-ANG II in cultured rabbit PTCs in the absence () or presence of the endocytotic inhibitor losartan (10 µM; ) or phenylarsine oxide (PAO; 1 µM; ). Endocytosis of [125I]Tyr-ANG II peaked at 30 min after exposure to the radioligand, which was significantly inhibited by losartan and PAO, suggesting an AT1 receptor-mediated response.

View larger version (76K): [in this window] [in a new window]   Fig. 3. Endocytosis of fluorescein-labeled ANG II (Fluo-ANG II) in the cytoplasm of cultured rabbit PTCs, where it colocalized with Alexa Fluor 594-labeled transferrin, an endosomal marker, 30 min after the cells were exposed to Fluo-ANG II. A: cytoplasmic localization of internalized Fluo-ANG II (green). B: nucleus stained with 4,6-diamidino-2-phenylindole (DAPI; blue). C: merged image of A and B, showing the relationship between Fluo-ANG II and the nucleus. D: Fluo-ANG II (green). E: endosomes stained with Alexa Fluor 594-labeled transferrin (red). F: merged image of D and E (yellow), showing colocalization of Fluo-ANG II and transferrin. Magnification, x40.

View larger version (17K): [in this window] [in a new window]   Fig. 4. Effects of AT1 and AT2 receptors on intracellular accumulation of extracellular ANG II in PTCs. Note that both the AT1 receptor blocker losartan (10 µM) and the AT2 receptor blocker PD-123319 (10 µM) inhibited intracellular ANG II accumulation, but the effect of losartan predominated. Los, losartan; PD, PD-123319. *P < 0.05; **P < 0.01 vs. control. +P < 0.05; ++P < 0.01 vs. ANG II. #P < 0.05 vs. ANG II + Los or ANG II + PD.

View larger version (13K): [in this window] [in a new window]   Fig. 5. Effects of endocytotic inhibitors on AT1 receptor-mediated accumulation of ANG II in PTCs. A: effects of cold (4°C), which inhibits AT1 receptor-mediated endocytosis, or sucrose (400 mM), which depletes clathrin-coated pits in non-renal cells. B: effects of the cytoskeleton microtubule inhibitor colchicine (1 µM) or the tyrosine phosphatase inhibitor PAO (1 µM). **P < 0.01 vs. control. ++P < 0.01 vs. ANG II.

View larger version (22K): [in this window] [in a new window]   Fig. 6. Effects of blockade of AT1-mediated ANG II endocytosis by losartan and PAO on basal intracellular cAMP responses to ANG II in PTCs. A: time-dependent inhibition of cAMP production by ANG II (1 nM), which peaked at 30 min. B: at 30 min, ANG II (1 nM) attenuated basal cAMP production and that losartan and PAO reversed ANG II-induced inhibition of basal cAMP production. *P < 0.05 vs. control. #P < 0.05 vs. ANG II.

View larger version (32K): [in this window] [in a new window]   Fig. 7. Effects of blockade of AT1-mediated ANG II endocytosis by losartan and PAO on forskolin-stimulated cAMP production in PTCs 30 min after exposure to the agonist and/or blockers. Note that forskolin stimulated cAMP production and ANG II (1 nM) significantly attenuated forskolin-stimulated cAMP production. Both losartan and PAO reversed ANG II-induced inhibition of forskolin-increased cAMP production, whereas PD-123319 did not. FKL, forskolin. *P < 0.05 vs. control. +P < 0.05 vs. ANG II. #P < 0.05 vs. FKL. &P < 0.05 vs. ANG II + FKL.

	DISCUSSION

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

The present study provides evidence that AT₁-mediated ANG II endocytosis plays an important role in high intracellular accumulation of ANG II in PTCs in vitro and, by implication, that this process also may occur in PTCs ex vivo. Investigators in our group and others have previously shown that circulating ANG II accumulates in the kidney of ANG II-infused rats via an AT₁-mediated mechanism(s) (36, 38, 42, 44); however, the cellular location of ANG II accumulation in the kidney as well as the mechanisms involved have not been determined. ANG II levels in the kidney are reportedly several thousand times higher than the circulating peptide, which leads to the hypothesis of compartmentalization of ANG II synthesis and/or release within the kidney (5, 23). Indeed, early studies reported nanomolar concentrations of ANG II in intrarenal fluid compartments, including the glomerular filtrate (31), proximal tubular fluid (5, 31), and renal cortical interstitial fluid (25, 32) compared with femto- to picomolar levels in the circulation. However, when van Kats et al. (35) infused ¹²⁵I-labeled ANG II into pigs and measured labeled peptide levels in different cellular fractions of the kidney homogenates, they found that most ¹²⁵I-ANG II is cell-associated due to AT₁ receptor-mediated endocytosis. We previously measured internalized AT_1A receptors and ANG II in isolated renal cortical endosomes and intermicrovillar clefts of ANG II-infused rats and found that AT_1A receptor antibody binding more than doubled, whereas ANG II levels were 5–10 times higher in endosomes and more than doubled in intermicrovillar clefts compared with control (42). Because coadministration of the AT₁ receptor blocker candesartan prevented accumulation of extracellular ANG II in endosomes and intermicrovillar clefts, we interpreted these findings as an AT_1A-mediated response. However, it should be emphasized that all previous studies were performed in whole kidney tissue, and therefore it is not possible to determine the cellular sites responsible for increased accumulation of extracellular ANG II in the kidney after long-term ANG II infusion.

In the present study, we used cultured rabbit PTCs as a tool to determine the contribution of AT₁-mediated endocytosis of extracellular ANG II to intracellular accumulation of ANG II and study the potential role(s) of clathrin-coated pits, cytoskeleton microtubules, and tyrosine phosphatases in AT₁-mediated ANG II accumulation in PTCs in vitro. Use of these cells as a model offers several advantages over the whole kidney approach in vivo. These cells express all necessary components of the RAS, including ANG II receptors, and respond to ANG II stimulation by activating intracellular signaling, commonly associated with PTC function (26, 27, 43). Although proximal tubules can be isolated for measurement of ANG II, the procedures are laborious and time-consuming, and the reagents used for isolation and purification would likely alter ANG II formation and degradation. The main disadvantage with using whole kidney homogenates is perhaps that it is not possible to study the cellular mechanisms involved beyond the role of AT₁ receptors. In the present study, we first demonstrated that AT₁ (equivalent to human AT₁ and rodent AT_1A) receptor proteins are expressed in these PTCs by Western blot, using rabbit anti-AT₁ receptor antibodies raised against the NH₂-terminal or cytosolic domains of the receptor (11, 17, 42) and an AT₁ receptor-selective siRNA. We then confirmed that incubating these cells with ¹²⁵I-ANG II induced 80% internalization of the peptide within 30 min of exposure and that this was blocked by losartan, pointing to an AT₁ receptor-mediated mechanism. This phenomenon has been demonstrated previously in OK cells transfected with AT_1A receptors, although basal and internalized ANG II were not measured (33). We therefore extended previous studies by measuring intracellular ANG II before and after exposure to extracellular ANG II to promote receptor-mediated endocytosis. On the basis of cell number and protein content per well and ANG II concentrations, we can estimate basal endogenous ANG II content in these cells as well as the relative contribution of AT₁-mediated endocytosis of extracellular ANG II to intracellular ANG II accumulation in PTCs. There are 10⁶ cells or 360 µg protein in each well of a six-well plate when they have grown to 80% confluence. The basal concentration of ANG II is close to 200–250 pg/mg protein, which gives a calculated basal ANG II content of 70–90 pg/10⁶ cells. Intracellular ANG II content would increase by 50–70% to 110–150 pg/10⁶ cells, primarily due to AT₁-mediated endocytosis.

Whether AT₂ receptors mediate ANG II endocytosis and its subsequent intracellular signaling is not known (7, 9, 16, 45). Hein et al. (16) showed that unlike AT₁ receptors, AT₂ receptors transiently or stably expressed in HEK-293 cells do not internalize when they are stimulated by ANG II. As shown in Figs. 1 and 4, however, we found that rabbit PTCs also express low levels of endogenous AT₂ receptors and that the AT₂ receptor antagonist PD-123319 partially inhibited intracellular accumulation of extracellular ANG II, suggesting that endogenous AT₂ receptors perhaps play a minor role in mediating ANG II endocytosis in rabbit PTCs. Indeed, AT₂ receptors have been reported to mediate different biological effects in various renal cells (7).

The cellular mechanisms that regulate AT₁ (or AT_1A) receptor-mediated endocytosis are complex and often cell type specific. There are two recognized pathways for GPCR endocytosis, the classic clathrin-dependent and non-clathrin-dependent pathways (1, 9, 28). The most commonly cited pathways for GPCR-mediated endocytosis include clathrin-coated pits, -arrestin and/or dynamin proteins, -adaptin, and G protein-coupled receptor kinases (1, 9, 28). Because discussion of the role(s) of individual pathways in AT_1A receptor-mediated endocytosis is beyond the scope of the present study, we focused on the potential role(s) of three important pathways in mediating intracellular ANG II accumulation in PTCs. Clathrin-coated pits or vesicles, interacting with -arrestin and/or dynamin proteins, are widely credited with endocytosis of epidermal growth factor (9, 35) and ₂-adrenergic receptors (9) and also with AT_1A receptors in CHO or HEK-293 cells stably transfected with the mutant receptors (16, 33). We questioned whether clathrin-coated pits play a role in AT₁-mediated ANG II accumulation in PTCs. Our group previously showed that in the ANG II-infused rat kidney, ANG II accumulated in renal cortical endosomes, where it colocalized with AT_1A receptors (42); yet we could not determine whether clathrin-coated pits play any role in intracellular trafficking of ANG II/AT₁ receptor complex to the endosomes in vivo. In the present study, we found that pretreating PTCs with hyperosmotic sucrose (400 mM), which is commonly used to deplete clathrin-coated pits (2, 9, 35), did not significantly prevent receptor-mediated intracellular accumulation of ANG II, suggesting that non-clathrin endocytic pathways may play an important role in PTCs. Non-clathrin endocytic pathways also can deliver molecules to classic endocytic compartments, such as endosomes, and to other intracellular compartments, such as the Golgi apparatus and endoplasmic reticulum (28). Schelling et al. (29) demonstrated that in cultured rat PTCs, blocking receptor-mediated endocytosis with the cytoskeleton microtubule inhibitor colchicine or PAO, a tyrosine phosphatase-selective inhibitor, completely eliminated apical ANG II-induced phospholipase C (PLC)-mediated intracellular inositol 1,4,5-trisphosphate (IP₃) signaling and ²²Na transport. In the present study, we demonstrated that colchicine and PAO completely prevented AT₁-mediated intracellular ANG II accumulation in PTCs, supporting the hypothesis that AT₁-mediated endocytosis of extracellular ANG II in PTCs is cytoskeleton microtubule-dependent and requires activation of tyrosine phosphatases.

How cytoskeleton microtubules or tyrosine phosphatases could modulate AT₁-induced intracellular accumulation of extracellular ANG II in PTCs remains to be determined. Cytoskeleton microtubules are polarized cytoplasmic structures extending from the perinuclear region toward the periphery of the cell (3, 6, 19). Cytoskeleton microtubules, acting through the dynein activator protein dynactin, play an important role in cytoplasmic trafficking of viruses, solutes, or proteins from early endosomes to late endosomes or lysosomes and from the endoplasmic reticulum to the Golgi apparatus inside mammalian cells (3, 6, 19). PTCs are polarized epithelial cells with their apical membrane facing the tubular lumen and their basolateral membrane touching the peritubular capillaries. Solutes, amino acids, peptides, and glucose are transported into cells via receptor-mediated endocytosis or by various transporters (3, 6, 21). It is likely that colchicine prevented intracellular ANG II accumulation by inhibiting cytoplasmic trafficking of the peptide after endocytosis. In VSMCs, disruption of cytoskeleton microtubules with nocodazole blocked AT₁ receptor trafficking into caveolae/lipid rafts (45). By contrast, PAO may block AT_1A-mediated ANG II endocytosis via a different mechanism. PAO is a general inhibitor of tyrosine phosphatases that has been widely used to study AT_1A receptor endocytosis (12, 30), but it is not clear which specific tyrosine phosphatase it inhibits and how it inhibits AT_1A receptor endocytosis. Previous studies have shown that PAO inhibits not only AT_1A receptor endocytosis (12, 30) but also other GPCR endocytosis (33, 36). Thus PAO may not act specifically at the receptor level and, instead, inhibits receptor endocytosis by targeting the endocytotic machinery such as arrestins, dynamins, or cytoskeleton microtubules. It is also likely that PAO may inhibit one of tyrosine phosphatases that play a role in GPCR endocytosis. Nevertheless, because PAO inhibits protein tyrosine phosphatases and therefore induces protein tyrosine dephosphorylation, our results suggest that tyrosine phosphatases and/or tyrosine dephosphorylation are involved in AT_1A receptor-mediated intracellular accumulation of extracellular ANG II in proximal tubule cells. Further studies are required to identify which specific protein tyrosine phosphatase regulates AT_1A receptor endocytosis and elucidate the cellular mechanisms involved.

Our results show that AT₁-mediated endocytosis of extracellular ANG II may play a functional role in regulating proximal tubular sodium transport. In the present study, increased intracellular accumulation of extracellular ANG II via AT₁ receptor-mediated endocytosis was associated with decreased basal and forskolin-stimulated intracellular cAMP production. Losartan and PAO inhibited AT₁-mediated ANG II endocytosis in PTCs, and both prevented the effects of ANG II on intracellular cAMP production, indicating that internalized ANG II does indeed play a functional role in PTC function. Alternatively, because coadministration of losartan or PAO with ANG II increased cAMP production to the levels that were significantly higher than control or ANG II alone (Fig. 6B), other mechanisms unrelated to AT₁-mediated ANG II endocytosis may be involved. There is evidence that receptor-mediated ANG II endocytosis is important not just for transporting the ligand to the lysosomes for destruction and recycling the receptors back to the cell surface and that receptor-mediated ANG II endocytosis may be important in regulating biological actions of ANG II in PTCs. Schelling et al. (29, 30) demonstrated that endocytosis of the ANG II-AT₁ receptor complex activated PLC-IP₃ signaling, increased sodium flux, and decreased cAMP signaling in cultured rat PTCs. Becker et al. (4) showed that AT₁ receptor-mediated endocytosis was associated with increased phospholipase A₂ activity and sodium flux in LLC-PK cells expressing rabbit AT₁ receptors. Thekkumkara and Linas (34) reported that in OK cells, apical membrane AT_1A receptors were internalized before they interact with G proteins, leading to inhibition of cAMP signaling. Accordingly, our finding that inhibition of AT₁ receptor-mediated endocytosis of extracellular ANG II blocked intracellular ANG II accumulation, and therefore ANG II-induced inhibition of cAMP signaling in PTCs, is consistent with these previous observations.

In summary, we have demonstrated in cultured rabbit PTCs, which express endogenous AT₁ receptors, that 1) intracellular ANG II levels increase significantly when cells are exposed to extracellular ANG II; 2) increased intracellular ANG II accumulation is inhibited by the AT₁ receptor antagonist losartan, the cytoskeleton microtubule inhibitor colchicine, or the tyrosine phosphatase inhibitor PAO; 3) depletion of clathrin-coated pits with hyperosmotic sucrose has no effect on intracellular ANG II accumulation; and 4) inhibition of AT₁ receptor-mediated intracellular ANG II accumulation blocks ANG II-inhibited cAMP production. These results suggest that AT₁ receptor-mediated endocytosis of extracellular ANG II in PTCs contributes to increased intrarenal ANG II accumulation in vivo and also plays a functional role in the regulation of proximal tubule cell function by regulating intracellular cAMP signaling.

	GRANTS

TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
This work was supported in part by National Institute of Diabetes and Digestive and Kidney Diseases Grant 5R01 DK-067299 (to J. L. Zhuo), American Heart Association Grant-in-Aid 0355551Z, and a National Kidney Foundation Grant-in-Aid. O. A. Carretero is supported by National Heart, Lung, and Blood Institute (NHLBI) Program Project Grant HL-28982. L. G. Navar is supported by NHLBI Grant HL-26371. Parts of this work were presented as an abstract at the Gordon Research Conference on Angiotensin in 2004 and the Federation of American Societies for Experimental Biology Summer Research Conference on Renal Microcirculatory and Tubular Dynamics in 2004.

	FOOTNOTES

 

Address for reprint requests and other correspondence: J. L. Zhuo, Division of Hypertension and Vascular Research, Henry Ford Hospital, 2799 West Grand Blvd., Detroit, MI 48202 (e-mail: jzhuo1{at}hfhs.org)

The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

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TOP ABSTRACT MATERIALS AND METHODS RESULTS DISCUSSION GRANTS REFERENCES

 

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