Distribution of Signaling Molecules Involved in Vasopressin-induced Ca2+ Mobilization in Rat Hepatocyte Multiplets

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ARTICLE

Distribution of Signaling Molecules Involved in Vasopressin-induced Ca²⁺ Mobilization in Rat Hepatocyte Multiplets

Dien Tran^a, Nicole Stelly^a, Thierry Tordjmann^a, Thierry Durroux^b, Marie Noelle Dufour^b, Arlette Forchioni^c, René Seyer^b, Michel Claret^a, and Gilles Guillon^b
^a INSERM U442, IFR-FR 46, Université Paris Sud, Orsay, France
^b INSERM U469 Université Montpellier I, Montpellier, France
^c Service d'Imagerie Cellulaire, Université Paris Sud, Orsay, France

Correspondence to: Michel Claret, Signalisation Cellulaire et Calcium, INSERM U442, IFR-FR 46, Université Paris Sud, bât. 443, 91405 Orsay, France.

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In freshly isolated rat hepatocyte multiplets, Ca²⁺ signalsin response to vasopressin are highly organized. In this studywe used specific probes to visualize, by fluorescence and confocalmicroscopy, the main signaling molecules involved in vasopressin-mediatedCa²⁺ responses. V1a receptors were detected with a novel fluorescentantagonist, Rhm⁸-PVA. The G ${alpha}$ q/G ${alpha}$ 11, PLCß₃, PIP₂, and InsP₃receptors were detected with specific antibodies. V1a vasopressinreceptors and PIP₂ were associated with the basolateral membraneand were not detected in the bile canalicular domain. G ${alpha}$ q/G ${alpha}$ 11,PLCß₃, and InsP₃ receptors were associated with the basolateralmembrane and also with other intracellular structures. We useddouble labeling, Western blotting, and drugs (cytochalasin D,colchicine) known to disorganize the cytoskeleton to demonstratethe partial co-localization of G ${alpha}$ q/G ${alpha}$ 11 with F-actin. (J HistochemCytochem 47:601–616, 1999)

Key Words: hepatocyte multiplets, fluorescent antagonist, V1a receptors,antibodies, G ${alpha}$ q/G ${alpha}$ 11, cytoskeleton, fluorescence and confocalmicoscopy, Western blotting

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The hepatocyte is a highly polarized epithelial cell. Its plasmamembrane consists of three morphologically and functionallydifferent regions: the basal domain, which is in contact withthe blood; the lateral domain, which segregates gap and tightjunctions; and the canalicular domain, which is involved inthe secretion of native bile (Keppler and Arias 1997 ). Thepreparation of isolated hepatocytes causes single cells to losetheir polarity and all the proteins originally segregated intothe various domains to become randomly redistributed throughoutthe plasma membrane. However, the cell suspension contains multiplets(e.g., doublets, triplets, quadruplets), small groups of cellsthat retain certain aspects of structural and functional polarity,particularly the three plasma membrane domains found in theintact liver (Gautam et al. 1987 ; Graf and Boyer 1990 ; Watanabeet al. 1991a ; Spray et al. 1994 ; Boyer 1997 ).

The hepatocyte doublet system has been used to demonstrate thatthe intracellular Ca²⁺ wave begins in the pericanalicular (apical)region and propagates peripherally (Nathanson et al. 1994a )as in exocrine acinar cells (Kasai et al. 1993 ; Thorn et al.1993 ; Tojyo et al. 1997 ). This subcellular Ca²⁺ wave organizationprobably results either from a higher density of the inositol1,4,5-trisphosphate (InsP₃) receptor in the pericanalicularregion (Nathanson et al. 1994a , Nathanson et al. 1994b ; Leeet al. 1997 ; Yule et al. 1997 ) or from a gradient in InsP₃receptor sensitivity across the cell, with the receptors atthe apical pole having higher affinity for InsP₃ than thoseat the basolateral area (Kasai et al. 1993 ; Thorn et al. 1993). Ca²⁺ waves and synchronized oscillations travel from cellto cell in hepatocyte doublets (Nathanson and Burgstahler 1992a, Nathanson and Burgstahler 1992b ; Boyer 1997 ), in multicellularsystems (Combettes et al. 1994 ; Tordjmann et al. 1997 , Tordjmannet al. 1998 ), and in the intact perfused liver (Nathanson etal. 1995 ; Robb-Gaspers and Thomas 1995 ). Cell doublet preparationshave been used to investigate a variety of cytoskeleton-dependentfunctions because the F-actin and tubulin networks remain polarizedin these preparations (Boyer 1997 ). The actin cytoskeletonis responsible for bile canalicular contraction (Watanabe etal. 1991a , Watanabe et al. 1991b ), which is itself stimulatedby increases in [Ca²⁺]_i (Oshio and Phillips 1981 ), cytosolicATP (Watanabe et al. 1991a ), or vasopressin concentrations(Kawahara and French 1990 ).

Here we investigated the subcellular localization of the signalingmolecules involved in vasopressin-mediated Ca²⁺ signals in multipletsof rat hepatocyte. This cellular model was used because themorphological and functional properties typical of liver tissuesare preserved. Thus, vasopressin-induced calcium oscillationhad been observed both on intact perfused liver (Nathanson etal. 1995 ; Robb-Gaspers and Thomas 1995 ) and on hepatocytemultiplets reported by our laboratory (Combettes et al. 1994; Tordjmann et al. 1997 , Tordjmann et al. 1998 ). Such studieshave been performed to improve our understanding of the spatiotemporalorganization of the vasopressin-stimulated calcium wave. Wefound that V1a vasopressin receptors and PIP₂ were located exclusivelyon the basolateral membrane, phospholipase Cß₃ (PLCß₃)was found, to a lesser extent, on the basolateral membrane andmainly on cytoplasmic structures, and ${alpha}$ q/ ${alpha}$ 11 G-protein subunits(G ${alpha}$ q/ G ${alpha}$ 11) and InsP₃ receptor were associated with both the basolateralmembrane and intracellular structures.

Materials and Methods

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Primary and Secondary Antibodies
The purified polyclonal antibody directed against the carboxyterminal decapeptide of G ${alpha}$ q/G ${alpha}$ 11 has previously been described(Ibarrondo et al. 1995 ). It is specific for G ${alpha}$ q/G ${alpha}$ 11 and inhibitsvasopressin-stimulated PLC activity. Because the carboxy terminaldecapeptide is common to ${alpha}$ q and ${alpha}$ 11 G-protein subunits, the antibodyrecognizes both molecules. The purified polyclonal antibodydirected against a 20-amino-acid C-terminal peptide from ratPLCß₃ was obtained from Santa Cruz Biotechnology (SantaCruz, CA). The specific mouse monoclonal antibody directed againstPIP₂ (IgG_2b subclass), has been described elsewhere (Fukamiet al. 1988 ; Tran et al. 1993 ). The polyclonal antibody directedagainst the whole Type 1 InsP₃ receptor molecule, purified fromsheep cerebellum, was produced and characterized in our laboratory.A single band was detected with this antibody on Western blots,and this band corresponded to the rat liver InsP₃ receptor.Therefore, this antibody was suitable for immunocytochemicalexperiments. It labeled the basolateral and canalicular domainsof hepatocytes on rat liver cryostat sections (Lievremont etal. 1996 ). The monoclonal anti- ${alpha}$ -tubulin antibody and the Cy3-labeledgoat anti-rabbit IgG were obtained from Amersham (ArlingtonHeights, IL). The polyclonal anti-actin antibody was purchasedfrom Sigma (St Louis, MO). FITC–anti-mouse IgG_2b was suppliedby Nordic Immunological Laboratories (Tilburg, The Netherlands),TRITC–anti-mouse IgG and biotinylated anti-rabbit IgG wereobtained from Jackson Immunoresearch Laboratories (West Grove,PA), and peroxidase-conjugated anti-rabbit and anti-mouse IgGwere purchased from Sanofi Diagnostics Pasteur (Marnes-la-Coquette,France).

Properties of the Fluorescent Vasopressin Antagonist of the V1a Receptor
A fluorescent vasopressin antagonist, 4-HO-Ph(CH₂)₂-CO-DTyr(Me)-Phe-Gln-Asn-Arg-Pro-Lys(5-carboxytetramethylrhodamyl]-NH₂(Rhm⁸-PVA), which binds to the V1a vasopressin receptor, hasbeen synthesized (Durroux et al. in press ). We used an antagonistto detect the cell surface V1a receptor because this preventedreceptor endocytosis (Lutz et al. 1992 ). Rhm⁸-PVA was synthesizedby coupling 5-carboxy tetramethyl rhodamine to a Lys⁸ linearvasopressin antagonist. The dissociation constant (K_i) of Rhm⁸-PVAwas 70 pM, as assessed by competition experiments with CHO cellsexpressing V1a receptors. Nonspecific binding accounted forno more than 20% of total binding for a concentration of Rhm⁸-PVAnear the K_i value. The K_i of Rhm⁸-PVA was 27 nM for V1b, 7490nM for V2, and 1.23 nM for oxytocin receptors. We also investigatedinhibition of the functional responses of V1a receptors by Rhm⁸-PVA.We found that Rhm⁸-PVA alone did not stimulate InsP₃ synthesis.It competitively inhibited the vasopressin-mediated synthesisof InsP₃ in CHO cells expressing V1a receptors with an inactivationconstant (Kinact) of 70 pM. (Durroux et al. in press ).

Preparation of Rat Hepatocytes
Single-cell and multicellular (doublets, triplets, quadruplets)hepatocyte systems were prepared by collagenase (BoehringerMannheim; Meylan, France) perfusion of liver from female Wistarrats (Janvier; Le Genest-St-Isle, France) as previously described(Combettes et al. 1986 ; Mauger et al. 1989 ). Isolated rathepatocytes were maintained (2 x 10⁶ cells/ml) at 22C in modifiedEagle's medium (MEM) (Gibco BRL Life Technologies; Paisley,UK) containing 1.5% gelatin (Labosi; Elancourt, France), throughwhich O₂/CO₂ (19/1) was continually bubbled. Cell viability,assessed by trypan blue exclusion, was over 96% for 4–5hr.

Cells (2.5 x 10⁵ cells/ml) were plated on collagen-coated glasscoverslips and incubated in Williams' medium E (Gibco) containing10% fetal calf serum, glutamine (2 mM), penicillin (100 U/ml),and streptomycin (100 µg/ml). They were incubated for2 hr at 37C under an atmosphere containing 5% CO₂ and 95% air.

Cells for treatment with cytochalasin D or colchicine were washedtwice with MEM containing 5 mM NaHCO₃, 20 mM Hepes, 1 g/literglucose, pH 7.4, and were incubated for 1 hr at 37C in thismedium with or without 2 µM cytochalasin D or 10 µMcolchicine (Sigma).

Detection of Rhm⁸-PVA Binding to the V1a Vasopressin Receptor in Rat Hepatocytes
Cells were rinsed twice and incubated for 15 min at 4C in MEMwith (autofluorescence and nonspecific binding) or without (autofluorescenceand total binding) 5 µM nonfluorescent antagonist V4253([ß-mercapto-ß-ß-cyclopenta-methylenepropionyl¹,O-Et-Tyr²,Val⁴,Arg⁸]-vasopressin) or 100 nM vasopressin (Sigma). The cellswere then incubated for 30 min at the same temperature with10 nM fluorescent antagonist, Rhm⁸-PVA, in MEM containing 1mg/ml bovine serum albumin (BSA) (Miles Laboratories; Kankakee,IL). Cells were washed twice with MEM at 4C, fixed by incubationfor 15 min with 4% formaldehyde (FA) (Merck; Darmstadt, Germany),and mounted in buffered glycerin (Sanofi Diagnostics Pasteur).In some experiments, fixed cells were further incubated withFITC–phalloidin (Sigma) (1 µg/ml) for 15 min at roomtemperature (RT) to label F-actin. Cells were then observedeither with an Axioskop epifluorescence photomicroscope (CarlZeiss; Le Pecq, France) equipped with a sensitive 3CCD-cooledcamera LH750RC3 (Lhesa; Cergy Pontoise, France) or with a confocalmicroscope (BIO-RAD MRC 600; Ivry-sur-Seine, France) equippedwith an argon–krypton mixed gas laser. The excitation wavelengthswere 546 nm for Rhm⁸-PVA and 490 nm for FITC–phalloidin.Images were processed using Photomat, Photoshop (epifluorescentmicroscope), or BIO-RAD (confocal microscope) software.

Immunodetection of G ${alpha}$ q/G ${alpha}$ 11, PLCß₃, PIP₂, the InsP₃ Receptor, Tubulin and F-actin by Fluorescence and Confocal Microscopy
Cells were fixed in 4% FA in PBS for 15 min at RT and storedin 0.4% FA at 4C or were fixed in acetone at -20C for 5 min,then air-dried and stored desiccated at -20C. FA fixation wasessential for labeling of PIP₂ and G ${alpha}$ q/G ${alpha}$ 11, whereas acetone fixationwas better for PLCß₃. Both techniques were suitable forthe InsP₃ receptor, tubulin, and F-actin.

One of three methods was used to permeabilize FA-fixed cells:(a) 0.1% Triton X-100 (Sigma) in PBS for 2 min; (b) acetone:PBS(1:1) for 5 min; or (c) freezing and thawing after incubationwith 1 M sucrose for cryoprotection (essential for PIP₂).

Cells were washed with PBS and nonspecific binding sites wereblocked by incubation for 15 min with 50 mM NH₄Cl, then fora further 15 min with PBS containing 0.5% ovalbumin (Sigma).Cells were incubated overnight at 4C with the specific primaryantibodies [anti-G ${alpha}$ q/G ${alpha}$ 11 1:100, anti-PLCß₃ 1:100, anti-PIP₂1:1000, anti-InsP₃ receptor (InsP₃R) 1:10 or anti-tubulin 1:400],then for 30 min to 1 hr with the appropriate secondary antibody(for details see figure legends). A second fixation step with4% FA was generally performed after incubation with the secondaryantibody to stabilize the immune complex. Cells were finallyincubated for 20 min with 0.1% sodium borohydride (Sigma) inPBS to reduce autofluorescence.

Negative controls were carried out systematically by omittingthe specific primary antibodies and, if possible, by incubatingthe primary antibodies with an excess (500- to 1000-fold molarexcess) of the corresponding antigen before use.

The cells were incubated with fluorescent secondary antibodiesor biotinylated secondary antibodies followed by FITC–streptavidin(Immunotech; Marseille, France). TRITC or FITC–phalloidin(Sigma) was used at a concentration of 0.5–1 µg/mlfor 5–15 min for detection of F-actin. This staining ofF-actin made it easier to identify the bile canaliculus betweenadjacent hepatocytes.

Cells were mounted using the Slow Fade-Light antifade kit (MolecularProbes; Leiden, The Netherlands) or buffered glycerin. Theywere then observed and the images recorded with epifluorescenceand confocal microscopes equipped with appropriate software,as described above.

Preparation of Subcellular Fractions of Rat Hepatocytes
Hepatocytes plated and incubated for 2 hr on collagen-coatedcoverslips were rinsed twice with 20 mM Hepes buffer, pH 7.4,containing 50 mM NaCl, 5.6 mM KCl, 1.2 mM NaH₂PO₄, 5.1 mM NaHCO₃,and were collected by scraping. The following steps were allperformed at 4C. The collected cells were suspended in homogenizationbuffer [10 mM Tris-HCl, pH 7.4, 1 mM EDTA, 1 mM PMSF, 10 µg/mlleupeptin, and 10 µg/ml aprotinin (Sigma)], subjectedto sonication four times for 10 sec each, and centrifuged at100,000 x g for 1 hr. The pellet, containing total cell membranes(M), was resuspended in homogenization buffer. Cytosolic proteins(Cy) in the supernatant were precipitated overnight at -80Cby adding 9 volumes of acetone and were collected by centrifugationat 21,000 x g for 6 min.

The cytoskeleton (CK) was prepared as described by Payrastreet al. 1991 . The scraped hepatocytes were recovered by rapidcentrifugation (1,500 x g, 1 min, RT). The pellet was extractedby incubation for 15 min at 4C with 0.5% Triton X-100 in 20mM Hepes buffer, pH 7.4, containing 50 mM NaCl, 1 mM EGTA, 1mM PMSF, 10 µg/ml leupeptin, and 100 µM orthovanadate.The extracted preparation was centrifuged at 12,000 x g for2 min at 4C and the pellet containing the cytoskeleton and itsassociated proteins was washed twice at 4C with a buffer ofthe same composition but devoid of Triton X-100, and then suspendedin 20 mM Hepes buffer.

All fractions were stored at -80C and their protein contentwas determined by the Bio-Rad protein assay reagent using BSAas a standard.

Western Blotting of G ${alpha}$ q/G ${alpha}$ 11, PLCß₃, F-actin, and Tubulin
Proteins (10–20 µg per lane) were resolved by SDS-PAGE(7.5% acrylamide for PLCß₃ and 13% for actin, tubulin,and G ${alpha}$ q/G ${alpha}$ 11) and transferred to nitrocellulose membranes. Blotswere incubated for 1 hr at 37C in blocking medium (PBS containing5% skimmed milk powder and 0.1% Tween-20). They were then incubatedfor 2 hr at RT with polyclonal anti-PLCß₃ (1:200), anti-G ${alpha}$ q/G ${alpha}$ 11(1:500), anti-F-actin (1:200), or monoclonal anti- ${alpha}$ -tubulin (1:1000)antibodies in the blocking medium. The blots were washed withPBS and incubated for 1 hr at RT with peroxidase-conjugatedanti-rabbit IgG or anti-mouse IgG (1:2000). Blots were washedwith PBS and detected using the ECL kit (Amersham).

Fluorescence Intensity Profiles for Signaling Molecules Involved in the Vasopressin Response
Digitized confocal images of signaling molecules labeled withfluorescent probes were used to generate a radial line fluorescenceintensity profile from the basal membrane to the nucleus usingMatrox MAGIC software. One profile per cell was obtained fora total of more than 20 cells from two or three separate hepatocytepreparations. Fluorescence intensity profiles were normalizedas a percentage of maximal fluorescence (arbitrary units) andwere averaged to form a mean profile. For the X-axis, pixelswere transformed into µm (1 pixel = 0.25 µm) andthe cell membrane was positioned at point O. For double labeling(G ${alpha}$ q/G ${alpha}$ 11–F-actin, G ${alpha}$ q/G ${alpha}$ 11–tubulin, InsP₃R–F-actin),pseudocolor images were generated from digitized confocal imagesby Photoshop software using green for FITC and red for TRITC.Red (F-actin or tubulin) and green images (G ${alpha}$ q/G ${alpha}$ 11 or InsP₃R)from double labeling experiments were superimposed. Fluorescenceintensity profiles from the basal membrane to the nucleus wereobtained as described above.

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Subcellular Distribution of the V1a Vasopressin Receptor as Detected by the Fluorescent Antagonist Rhm⁸-PVA
We used a new specific fluorescent vasopressin antagonist, Rhm⁸-PVA(Durroux et al. in press ), to detect cell surface V1a receptorsin rat hepatocytes in the absence of any receptor-mediated internalization(Lutz et al. 1992 ).

Rhm⁸-PVA bound to the surface of rat hepatocytes (Figure 1A).There was also significant labeling within the cell, probablydue to the high autofluorescence of rat hepatocytes (Berthonet al. 1984 ) because cells incubated without Rhm⁸-PVA werealso labeled (Figure 1B and Figure 1D). The labeling aroundthe periphery of rat hepatocytes with Rhm⁸-PVA was specificand was prevented if rat hepatocytes were first treated for15 min at 4C with either 100 nM vasopressin or 5 µM nonfluorescentvasopressin antagonist (Tran et al. in press ). Confocal images(Figure 1C and Figure 1D) confirmed the results obtained byepifluorescence microscopy. There was a thin layer of peripheralspecific labeling presumably corresponding to the plasma membrane.The basolateral membranes of all hepatocyte multiplets examinedwere labeled (Figure 1B; Table 1). In contrast, in double labeling,the bile canaliculi that were strongly labeled for F-actin werenot labeled with Rhm⁸-PVA (Figure 1E and Figure 1F).

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Figure 1. Detection of V1a vasopressin receptors using the fluorescent specific antagonist Rhm⁸-PVA. Hepatocyte multiplets cultured for 2 hr on collagen-coated coverslips were incubated as described in Materials and Methods with (A,C) or without (B,D) 10 nM Rhm⁸-PVA. The cells were washed, fixed with 4% FA, and observed under an epifluorescence microscope (A,B) and a confocal microscope (C,D). Specific signals for the V1a vasopressin receptor were detected at the basal (large arrows) and lateral (small arrows) membranes. Intracellular autofluorescence was evident in control cells not incubated with Rhm⁸-PVA (B,D). In double labeling (E,F, epifluorescence microscope), the bile canalicular membrane (double arrows) was not labeled with Rhm>⁸- PVA (E) but was intensely stained by FITC–phalloidin (F). Images are representative of 54 cells and 26 bile canaliculi examined from three separate experiments. Bar = 10 µm.

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Table 1. Subcellular distribution of cytoskeleton and signaling molecules of the vasopressin pathway in rat hepatocytes^a

Subcellular Immunodetection of ${alpha}$ q/ ${alpha}$ 11 G-protein Subunits
The polyclonal anti-G ${alpha}$ q/G ${alpha}$ 11 antibody used in this study was characterizedin WRK₁ cells (Ibarrondo et al. 1995 ), in which it recognizedonly two bands, one of 42 kD and the other of 43 kD, in a fractionof rat hepatocyte plasma membrane and in a preparation of purifiedG ${alpha}$ q/G ${alpha}$ 11 from rat liver. This antibody has been shown to be suitablefor immunocytochemistry experiments (Ibarrondo et al. 1995 ).Epifluorescence images showed that the antibody labeled weaklythe basal membrane and more intensely the lateral membrane.Some intracellular structures were also labeled (Figure 2A).These labelings were better illustrated by confocal microscopy(Figure 2C). The labeled area was broader and more intense belowthe lateral and bile canalicular membranes than for the basalmembrane. This peripheral and intracellular labeling was notdetected if the specific primary antibody was preincubated withan excess of peptide antigen (Figure 2B) or was omitted (Figure2D). We examined more than 125 multiplets and found that 89%of basolateral and bile canalicular domains were labeled bythe anti-G ${alpha}$ q/G ${alpha}$ 11 antibody (Table 1).

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Figure 2. Subcellular distribution of ${alpha}$ q/ ${alpha}$ 11 G-protein subunits. Hepatocyte multiplets were grown as previously described, fixed with 4% FA, permeabilized with Triton X-100, and incubated with (A,C) or without (D) spe-cific anti-G ${alpha}$ q/G ${alpha}$ 11 antibodies (1/100) or with specific antibodies exhausted by an excess of peptide antigen (B). The cells were washed and incubated with biotinylated anti-rabbit IgG (1:200), then with FITC–streptavidin (1:500). The cells were then fixed again with 4% FA. (A,B) Images from the epifluorescence microscope. (C,D) Images from the confocal microscope. Labeling is significant in the cytoplasm, weak but detectable at the basal membrane (large arrows), more intense at the lateral membrane (small arrows) and under the bile canaliculi (double arrows). Images are representative of 367 cells examined from six separate experiments. Bar = 10 µm.

Association of ${alpha}$ q/ ${alpha}$ 11 G-protein Subunits with F-actin and Tubulin
G ${alpha}$ q/G ${alpha}$ 11 is associated with the cellular cytoskeleton of manycell lines (Cote et al. 1997b ; Ibarrondo et al. 1995 ), sowe performed double labeling experiments (G ${alpha}$ q/G ${alpha}$ 11–F-actinand G ${alpha}$ q/G ${alpha}$ 11–tubulin) to investigate the effect of drugsknown to disorganize the actin or tubulin networks on G ${alpha}$ q/G ${alpha}$ 11distribution in rat hepatocyte multiplets. Anti-G ${alpha}$ q/G ${alpha}$ 11 antibodies,biotinylated anti-rabbit IgG, and FITC–streptavidin wereused to detect G ${alpha}$ q/G ${alpha}$ 11 (Figure 3B) and TRITC–phalloidinto detect F-actin (Figure 3A). There was clear but partial co-localizationof F-actin and G ${alpha}$ q/G ${alpha}$ 11. Both were detected under the bile canaliculusand basolateral membranes. Intracellular labeling for F-actinand G ${alpha}$ q/G ${alpha}$ 11 was less intense. Cytochalasin D treatment stronglyaffected the actin network in both the basolateral membraneand bile canaliculus domains (Figure 3C), with no consistentperipheral labeling. Separate aggregates were labeled for F-actin.Cytochalasin D treatment also disorganized G ${alpha}$ q/G ${alpha}$ 11 labelings(Figure 3D). However, co-localization of these two moleculeswas preserved, their distributions being almost identical. Theeffect of cytochalasin D on F-actin and G ${alpha}$ q/G ${alpha}$ 11 distributionwas specific, with no change in tubulin labeling observed (notshown). The close association of G-proteins and actin filamentswas confirmed by biochemical experiments (see Figure 5). Inthe total cell membrane fraction, G ${alpha}$ q/G ${alpha}$ 11 and actin were detectedby Western blotting. By contrast, only G ${alpha}$ q was present with actinin the cytoskeleton fraction. G ${alpha}$ 11 was not detected even if wedoubled the amount of proteins.

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Figure 3. Effects of cytochalasin D treatment on G ${alpha}$ q/G ${alpha}$ 11 and F-actin subcellular distribution. Hepatocyte multiplets grown on coverslips were incubated with (C,D) or without (A,B) 2 µM cytochalasin D for 60 min at 37C. They were then fixed, permeabilized, and labeled for G ${alpha}$ q/G ${alpha}$ 11 with FITC–streptavidin as described in the legend to Figure 2. F-actin was labeled with TRITC–phalloidin (1 µg/ml). TRITC (F-actin; A,C) and FITC (G ${alpha}$ q/G ${alpha}$ 11; B,D) labeling was analyzed by confocal microscopy; basal membrane (large arrow), lateral membrane (small arrow), and bile canaliculi (double arrows). Images were representative of 80 cells examined from four separate experiments. Bar = 10 µm.

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Figure 4. Effects of colchicine treatment on G ${alpha}$ q/G ${alpha}$ 11 and tubulin subcellular distribution. Hepatocyte multiplets grown on coverslips were incubated for 60 min at 37C with (C,D) or without (A,B) 10 µM colchicine. They were then fixed and permeabilized as described in the legend to Figure 2. The cells were washed and incubated with a mixture of rabbit anti-G ${alpha}$ q/G ${alpha}$ 11 antibody (1:100) and mouse anti-tubulin antibody (1:400). They were incubated with biotinylated anti-rabbit IgG (1:200), then with a mixture of FITC–streptavidin (1:500) and TRITC anti-mouse IgG (1:100). TRITC (tubulin; A,C) and FITC (G ${alpha}$ q/G ${alpha}$ 11; B,D) labeling was analyzed by confocal microscopy. Images are representative of 75 cells examined from three separate experiments. Bar = 10 µm.

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Figure 5. Immunoblot analysis of hepatocyte subcellular fractions using anti-phospholipase Cß₃, anti-tubulin, anti-actin, and anti-G ${alpha}$ q/G ${alpha}$ 11 antibodies. Proteins from cytoskeleton (CK), cytosol (Cy), and total membrane (M) fractions (10 µg/lane) were resolved by SDS-PAGE, transferred to nitrocellulose and probed with antibodies directed against phospholipase Cß₃ (PLC), tubulin (Tub), actin (Act), and G ${alpha}$ q/G ${alpha}$ 11 as described in Materials and Methods. Results are representative of two to four experiments from two separate cell preparations. Mr, molecular weight.

Double labeling for tubulin and G ${alpha}$ q/G ${alpha}$ 11 was performed in rathepatocyte multiplets. The specific anti- ${alpha}$ -tubulin antibody labeledthe typical filamentous tubulin network, which was abundantin regions near the nucleus and around the bile canaliculi (Figure4A). Sparse punctate labeling of the tubulin network, was detectedassociated with the basolateral membrane areas (Figure 4A),in contrast to the continuous labeling of G ${alpha}$ q/G ${alpha}$ 11 proteins (Figure4B). In contrast, tubulin and G ${alpha}$ q/G ${alpha}$ 11 were both located underthe bile canaliculus membrane (96% of 43 bile canaliculi observed).Prior treatment with colchicine (10 µM for 1 hr at 37C)completely disrupted the intracellular microtubule network andsignificantly reduced the labeling in the bile canalicular area(Figure 4C). This colchicine effect was specific because nochange in the F-actin labeling was observed (not shown). Thelabeling of G ${alpha}$ q/G ${alpha}$ 11 in the basolateral membrane and cytoplasmwas not affected by colchicine treatment, but the treatmentdid reduce labeling around the bile canaliculus area (90% ofbile canaliculi observed) (Figure 4D). On Western blots (Figure5), G ${alpha}$ q/G ${alpha}$ 11 and tubulin were detected in the total membrane andcytoskeleton fractions. In contrast, tubulin was abundant inthe cytosolic fraction in which G ${alpha}$ q/G ${alpha}$ 11 was not detected.

Subcellular Distribution of PLCß₃
The antibody used to detect PLCß₃ in rat hepatocytes wasspecific. On Western blots, it recognized only one band, witha molecular weight (152 kD) corresponding to that of PLCß₃(Figure 5). PLCß₃ was present mostly in the cytosol andthe total membrane fractions after cell fractionation. It wasnot detected in the cytoskeleton preparation. Immunofluorescenceexperiments showed similar results. There was heterogeneouslabeling of vesicles in the cytoplasm, mainly under the basalmembrane as shown by optical sections at a tangent to the cellsurface (Figure 6A). To a lesser extent, labeling vesicles werealso associated with the plasma membrane in equatorial sections(Figure 6B). The nuclear area was not specifically labeled,whereas an intense signal was obtained with an antibody directedagainst PLCß₁ (UBI; Lake Placid, NY) in rat hepatocytes(not shown). All labeling was abolished if the primary antibodywas omitted from the first incubation medium or if it was incubatedbefore the experiment with an excess of the antigen used toproduce it (Figure 6C). More than 100 cells were examined andno labeling was observed near the bile canaliculi (Table 1).

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Figure 6. Subcellular distribution of phospholipase Cß₃. Hepatocyte multiplets grown on coverslips were fixed with acetone and incubated with specific rabbit anti-phospholipase Cß₃ antibody (1:100) (A,B). The cells were washed and incubated with Cy3 anti-rabbit IgG (1:1000). Cy3 labeling was analyzed by confocal microscopy. (A) Optical section at a tangent to the cell surface, showing many fluorescent vesicles. (B) Equatorial section of the same cell group shown in A. The fluorescent vesicles were associated with the cell membrane (arrows) and the cytoplasm under the cell membrane. (C) Control with specific primary antibody exhausted by an excess of the antigen. Images are representative of 250 cells examined from three separate experiments. Bar = 10 µm.

Subcellular Distribution of Phosphatidyl Inositol 4,5-bisphosphate
We used the previously characterized specific antibody directedagainst PIP₂ (Fukami et al. 1988 ; Tran et al. 1993 ) to showthat the substrate of PLCß₃ was primarily associated withthe basal membrane, with labeling clustered in intense patches(Figure 7B). All cells examined were labeled in this heterogeneousmanner (Table 1). The control rat hepatocytes incubated in theabsence of primary antibody were not labeled (Figure 7D). PIP₂was not detected in the lateral and bile canaliculus membranes,whereas these areas were extensively labeled with F-actin (Figure7A).

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Figure 7. Subcellular distribution of PIP₂. Hepatocyte multiplets grown on coverslips were fixed with 4% FA, permeabilized by the freeze–thaw technique (see Materials and Methods), and incubated with (B) or without (D) anti-PIP₂ antibody (1:1000). The cells were fixed again with 4% FA to stabilize the antigen–antibody complex, then washed and incubated with FITC–anti-mouse IgG_2b (1:100) and TRITC–phalloidin (1 µg/ml). TRITC (F-actin; A) and FITC (PIP₂;B) labeling was analyzed by confocal microscopy. Control without TRITC–phalloidin (C); control without anti-PIP₂ antibody (D). Images are representative of 200 cells examined from five independent experiments. Bar = 10 µm.

Subcellular Distribution of the InsP₃ Receptor
The polyclonal antibody used in this study was directed againstthe entire InsP₃ receptor isoform 1 molecule purified from sheepcerebellum. This antibody recognized only one band of 260 kDin a plasma membrane-rich preparation of rat hepatocytes andwas shown to be suitable for immunocytochemical experiments(Lievremont et al. 1996 ). The anti-InsP₃R antibody labeledboth the basolateral membrane and the bile canalicular domainwith almost the same intensity (see Table 1). An intracellularnetwork near the membrane was also labeled (Figure 8A). Controlsnot incubated with the primary antibody were not labeled (Figure8B). Partial co-localization of the InsP₃ receptor and F-actinwas observed at the basolateral membrane and around the bilecanaliculi (Figure 8C and Figure 8D).

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Figure 8. Subcellular distribution of the InsP₃ receptor. Hepatocyte multiplets grown on coverslips were fixed with 4% FA, permeabilized with PBS: acetone (1:1), and incubated with (A) or without (B) rabbit anti-InsP₃R antibody (dilution 1:10). The cells were washed and incubated with biotinylated anti-rabbit IgG (1:200) and then with FITC–streptavidin (1:500). They were then fixed again with 4% FA and analyzed by confocal microscopy. Double labeling: FITC–labeled InsP₃R (C) and TRITC-labeled F-actin (D) showed partial co-localization of the two molecules; basal membrane (arrow) and bile canaliculi (double arrows). A is representative of 181 cells examined from six separate experiments. Bar = 10 µm.

Discussion

Top
Summary
Introduction
Materials and Methods
Results
Discussion
Literature Cited

The cellular response to a given hormonal stimulus depends onmany factors, the most important of which is the molecular equipmentof the cell. Thus, for the hormonal G-protein-coupled receptors(GPCRs), the cell's specific patterns of response and regulationdepend on the hormonal receptor subtype, the combination ofheterotrimeric G-protein subunits (Kleuss et al. 1993 ; Macrez-Lepretreet al. 1997 ), and the isoform of adenylyl cyclase or phospholipaseC (Jhon et al. 1993 ; Boyer et al. 1994 ; Kim et al. 1997). The subcellular distribution of the transducing moleculesmay also be important. For example, aquaporin-3 (AQP3) is constitutivelyexpressed at the basolateral membrane of renal collecting ductcells (Ecelbarger et al. 1995 ) and AQP2 is predominantly presentin subapical vesicles which, on activation of the V2 receptorwith vasopressin, fuse with the apical membrane (Nielsen etal. 1995 ). Similarly, in rat hepatocytes, receptors for epidermalgrowth factor, low-density lipoproteins, asialoglycoproteins,and insulin are concentrated at the basolateral membrane, whereasmany enzymes, such as 5' nucleotidase, dipeptidylpeptidase IV,aminopeptidase N, and ecto ATP^ase HA₄, are located at the apicalmembrane (Hubbard et al. 1994 ). The transduction mechanismstriggered by GPCRs involve several different molecules. We thereforedecided to investigate the subcellular distribution of thesemolecules in freshly isolated rat hepatocyte multicellular systemsbecause these multiplets retain some of the structural and functionalproperties of liver tissue (Gautam et al. 1987 ; Graf and Boyer1990 ; Watanabe et al. 1991a ; Spray et al. 1994 ; Boyer1997 ). Furthermore, rat hepatocytes have been extensively usedfor analyzing vasopressin-induced calcium signals, which areorganized as directional intracellular and intercellular waves(Rooney et al. 1990 ; Nathanson and Burgstahler 1992a , Nathansonand Burgstahler 1992b ; Combettes et al. 1994 ; Thomas etal. 1996 ; Tordjmann et al. 1997 , Tordjmann et al. 1998 ).We used a new fluorescent vasopressin receptor probe, Rhm⁸-PVA(Durroux et al. in press ), specific antibodies directed againstthe molecules of the vasopressin transduction pathway (Fukamiet al. 1988 ; Tran et al. 1993 ; Ibarrondo et al. 1995 ; Lievremont et al. 1996 ), and accurate confocal microscopy techniquesto determine the distribution of vasopressin-linked signalingmolecules in rat hepatocyte multicellular systems.

The principal molecules involved in the generation of vasopressin-stimulatedcalcium waves were not evenly distributed within the cells (Table1, Figure 9 and Figure 10). The V1a receptor detected withRhm⁸-PVA was associated with the basolateral membrane and wasabsent from the bile canaliculi and cytoplasm. PhospholipaseCß₁ interacts with the ${alpha}$ q/ ${alpha}$ 11 G-protein (Taylor et al. 1991; Jhon et al. 1993 ; Blank 1996 ; Piiper et al. 1997 ; Rheeand Bae 1997 ) and therefore with the V1a receptor because theseG-protein subunits have been reported to bind to this vasopressinreceptor subtype (Wange et al. 1991 ; Jhon et al. 1993 ; Thibonnieret al. 1993 ; Offermanns et al. 1994 ; Strakova et al. 1997). A commercial specific antibody against this PLC isoform didnot recognize the expected band in Western blot analysis oftotal membrane and cytosol fractions from rat hepatocytes. Theplasma membrane was weakly labeled and the perinuclear and nuclearregions strongly labeled, as previously observed for these cells(Divecha et al. 1993 ) and 3T3 cells (Zini et al. 1993 ). Forall these reasons, we focused on PLCß₃, which also interactswith ${alpha}$ q/ ${alpha}$ 11 G-protein subunits (Jhon et al. 1993 ; Blank 1996; Rhee and Bae 1997 ; Piiper et al. 1997 ) and therefore withthe V1a receptor. This isoform was associated with small vesiclesin the cytoplasm near the basolateral membrane but was absentfrom the bile canalicular area. It was detected in the cytosoland total membrane fractions, as demonstrated by Western blotting(Figure 5). Preliminary results showed that, on vasopressinstimulation, PLCß₃ was translocated from cytoplasmic structuresto the basolateral membrane (unpublished results). This suggeststhat the V1a receptor is functionally coupled to the PLCß₃isoform in rat hepatocytes. Such a translocation of PLCß₃has been reported in human platelets on thrombin stimulation(Banno et al. 1996 ). PIP₂ also had a heterogeneous distribution.It was found exclusively in patches associated with the basalplasma membrane. By different experimental approaches, the compartmentalizationof PIP₂ has been reported in many cell lines, including A431(Pike and Casey 1996 ), MDCK (Hope and Pike 1996 ), and Neuro2a (Liu et al. 1998 ). This suggests that such a heterogeneouslabeling could not arise from a fixation artifact. In contrast,the distribution of G ${alpha}$ q/G ${alpha}$ 11 and InsP₃ receptors is more homogeneous.Both are associated with the plasma membrane and the cytoskeleton(Bourguignon et al. 1993 ; Feng and Kraus-Friedmann 1993 ; Kraus-Friedmann 1994 ; Ibarrondo et al. 1995 ; Lievremontet al. 1996 ; Cote et al. 1997b ) or vesicles called caveoles(Fujimoto et al. 1992 ). Nathanson et al. 1994a demonstratedthat calcium waves induced by vasopressin originate from theapical pole (bile canaliculus) and propagate to the basolateraldomain. They also demonstrated a higher density of InsP₃ receptorsat the apical pole of the rat hepatocyte couplet. Our studyshowed that the density of InsP₃ receptors is similar in thebasolateral and bile canaliculus domains of the rat hepatocyte(Figure 8). These different data are consistent with both aheterogeneous density of InsP₃ receptors and a gradient of InsP₃receptor sensitivity across the hepatocyte. The receptors atthe basal pole may have a low affinity for InsP₃ and may thereforenot be activated by locally produced InsP₃. The InsP₃ receptorsat the apical pole may have a high affinity for InsP₃ diffusingfrom the basal pole, as suggested for pancreatic acinar cells(Kasai et al. 1993 ; Thorn et al. 1993 ) and parotid acinarcells (Tanimura et al. 1998 ).

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Figure 9. Distribution of vasopressin signaling molecules within the rat hepatocyte multiplets. The molecules involved in the generation of the calcium wave induced by vasopressin are represented in the various domains of a hepatocyte doublet. In this figure, the size of each molecule in a given area is proportional to its relative abundance.

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Figure 10. Normalized fluorescence intensity profiles of signaling molecules involved in the vasopressin response. The V1a vasopressin receptor (V1aR), ${alpha}$ q/ ${alpha}$ 11 G-protein subunits (G ${alpha}$ q/ ${alpha}$ 11), phospholipase Cß3 (PLCß₃), phosphatidyl inositol 4,5-bisphosphate (PIP₂), and InsP₃ receptor (InsP₃R) from rat hepatocytes, were labeled using fluorescent specific analogues or specific antibodies as described in Table 1. Digitized confocal images of signaling molecules were analyzed to obtain the fluorescence intensity profile from the basal membrane towards the nucleus using Matrox MAGIC software (see Materials and Methods). Results were normalized as a percentage of the peak fluorescence value (arbitrary units) for each signaling molecule profile. Data presented are the means of over 20 profiles per signaling molecule (one profile/cell) from two or three separate hepatocyte preparations. The dotted line from the fluorescence intensity profile of V1aR represents autofluorescence (cells incubated without the specific fluorescent antagonist). In all other cases, correction was made for autofluorescence by adjusting the origin for the Y-axis.

Transducing molecules may also be rapidly redistributed withinthe hepatocyte, from the basolateral pole to the bile canaliculus,during hormonal stimulation. Such a redistribution has beendescribed for V1a and V2 vasopressin receptors in A7r5 and A10smooth muscle and LLC-PK1 cell lines (Jans et al. 1989 , Janset al. 1990 ; Lutz et al. 1990 ), for ${alpha}$ -subunits of G-proteins(Ransnas et al. 1989 ; Svoboda and Milligan 1994 ; Banno etal. 1996 ; Cote et al. 1997a , Cote et al. 1997b ; Corneaet al. 1998 ), and for PLC (Yang et al. 1994 ; Banno et al.1996 ). Experiments are now under way to investigate whethersuch a redistribution occurs in rat hepatocytes.

Previous studies have demonstrated the involvement of the cytoskeletonin the transduction mechanisms involving GPCRs. Drugs, suchas cytochalasin D and colchicine, which disorganize actin ortubulin networks, inhibit second messenger production in a varietyof cell types, including rat adrenal glomerulosa (Cote et al.1997a , Cote et al. 1997b ) and WRK1 cells (Ibarrondo et al.1995 ). They also reduce hormonal responses, such as steroidogenesisin frog adrenocortical cells (Feuilloley et al. 1993 ; Feuilloleyand Vaudry 1996 ) and albumin secretion in rat hepatocytes (Saucanand Palade 1991 ). These effects probably arise from close interactionsbetween transducing molecules and the cellular cytoskeleton.Thus, G-proteins subunits such as ${alpha}$ i, ${alpha}$ q, ${alpha}$ 11, ${alpha}$ s, ß, or ${gamma}$ 12have been found to be associated with actin and/or tubulin networks(Carlson et al. 1986 ; Sarndahl et al. 1993 ; Ibarrondo etal. 1995 ; Cote et al. 1997a , Cote et al. 1997b ; Ueda etal. 1997 ). PLCß₃ and protein kinase C interact with thecytoskeleton in a cytochalasin D-dependent manner (Banno etal. 1996 ). Similar interactions were expected in rat hepatocytesbecause, first, cytochalasins B and D affect bile canalicularcontractions (Phillips et al. 1983 ; Watanabe et al. 1991b; St Pierre et al. 1997 ) and decrease bile flow but do notaffect the biliary secretion of organic anions (St Pierre etal. 1997 ). Colchicine inhibits the uptake, transport and secretionof horseradish peroxidase (Kono et al. 1997 ) second, hormonalreceptors involved in the regulation of hepatocyte functions,such as the V1a vasopressin, AT_1A angiotensin II, ${alpha}$ 1 adrenergic,and P_2Y purinergic receptors, are coupled to PLC via ${alpha}$ q/ ${alpha}$ 11 G-proteins(Wange et al. 1991 ; Jhon et al. 1993 ; Thibonnier et al.1993 ; Offermanns et al. 1994 ) that are associated with theactin and/or tubulin networks (Ibarrondo et al. 1995 ; Coteet al. 1997b ). This study clearly demonstrates that ${alpha}$ q/ ${alpha}$ 11 G-proteinsare associated with the cytoskeleton, presumably particularlywith actin filaments in rat hepatocytes because (a) cytochalasinD treatment disorganizes both F-actin and G ${alpha}$ q/G ${alpha}$ 11 labeling, whereascolchicine does not (Figure 3), (b) Western blot analysis showedthat G ${alpha}$ q was associated with an actin-rich Triton X-100-insolublecytoskeleton preparation (Figure 5), and (c) F-actin and G ${alpha}$ q/G ${alpha}$ 11double labeling gave similar profiles (Figure 11A) for bothmolecules, whereas double labeling with tubulin and G ${alpha}$ q/G ${alpha}$ 11 didnot (Figure 11B). These data are consistent with results obtainedwith WRK1 cells (Ibarrondo et al. 1995 ) and rat adrenocorticalcells (Cote et al. 1997b ) but conflict with those showing apreferential association of the tubulin network with G ${alpha}$ q in Sf9cells (Popova et al. 1997 ), and with G ${alpha}$ s and G ${alpha}$ i in rat cerebralcortex synaptic membranes (Wang et al. 1990 ). The distributionsof F-actin and G ${alpha}$ q/G ${alpha}$ 11 were not identical, however (Figure 11A),so we cannot exclude the possibility that G ${alpha}$ q/G ${alpha}$ 11 also interactswith tubulin or other intracellular filaments, as observed inrat adrenocortical cells (Cote et al. 1997b ). Therefore, theassociation of G ${alpha}$ q/G ${alpha}$ 11 with cytoskeleton fibers appears to bea general phenomenon but its functional significance is unknown.Actin filaments rapidly depolymerize and repolymerize on hormonalstimulation (Rijken et al. 1991 ; Norman et al. 1994 ). Theymay therefore regulate the coupling of calcium-mobilizing hormonereceptors and G ${alpha}$ q/G ${alpha}$ 11. Remodeling of actin cytoskeleton networksmay thus alter the generation of second messengers and regulatethe physiological effects associated with GPCRs.

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Figure 11. Fluorescence intensity profiles of cytoskeleton and signaling molecules. Double labeling of F-actin (Act) and tubulin (Tub) networks with either ${alpha}$ q/ ${alpha}$ 11 G-protein subunits (G ${alpha}$ q/G ${alpha}$ 11) (A,B) or the InsP₃R (C) was performed as described in the legends to Figure 3 and Figure 4. Pseudocolor images were generated from digitized confocal images by Photoshop software using green for FITC and red for TRITC. Red images (Act or Tub) and green images (G ${alpha}$ q/G ${alpha}$ 11 or InsP₃R) were superimposed. Fluorescence intensity profiles from the basal membrane to the nucleus were obtained using Matrox Magic software. Results were normalized as a percentage of the peak fluorescence value for each profile. Data presented are the means of more than 20 profiles (one profile/cell) for each molecule studied from two separate hepatocyte preparations. Autofluorescence level (omission of specific primary antibodies and TRITC–phalloidin) corresponds to point zero on the Y-axis.

Further evidence for the involvement of the cytoskeleton inhepatocyte signal transduction is provided by the followingfacts. (a) Both F-actin and V1a receptor-specific labeling areconcentrated (Figure 10 and Figure 11A) and co-localized (resultsnot shown) in the basolateral membrane. (b) InsP₃ receptorsare associated with cytoskeleton structures in the liver (Fengand Kraus- Friedmann 1993 ) and in human platelets (Bourguignonet al. 1993 ) and are functionally sensitive to drugs that affectcytoskeleton structure (Bourguignon et al. 1993 ). This studyalso showed partial co-localization of the InsP₃ receptor andthe F-actin network in rat hepatocytes (Figure 11C).

We also found a difference in the distribution of the two ${alpha}$ G-proteinsubunits studied. The plasma membrane contained both ${alpha}$ q and ${alpha}$ 11but in unequal proportions (73 ± 4 and 27 ± 4%respectively). The cytoskeleton fraction contained only the ${alpha}$ q-subunit (M_r 42 kD). The ${alpha}$ 11 band was undetectable even if theamount of cytoskeleton proteins in the gel well was increased(Figure 5). This is one of the first examples of a cell preparationexhibiting only the ${alpha}$ q G-protein subunit. However, the significanceof this is unclear. It may reflect a preferential coupling ofthe V1a vasopressin receptor and the ${alpha}$ q G-protein subunit inrat hepatocytes. Indeed, only the receptor-coupled G-proteinsubunit can be phosphorylated on hormonal stimulation, as previouslyobserved in a transfected CHO cell line (Umemori et al. 1997). Therefore, only this G-protein can interact in its phosphorylatedform with the cytoskeleton, as previously observed by Bannoet al. 1996 . Specific antibodies directed against ${alpha}$ q or ${alpha}$ 11 G-proteinsare required to test this hypothesis. Unfortunately, none ofthe available antibodies is suitable for immunocytochemicalstudies (unpublished results).

This study has determined the subcellular distribution of allthe main transducing molecules involved in vasopressin signalingin the rat hepatocyte. Experiments are now in progress to studythe translocation of signaling molecules from one compartmentto another on hormonal stimulation, to improve our understandingof the hormonal signals in the liver.

Acknowledgments

We would like to thank R. Leuillet for excellent hepatocytepreparations, D. Villette for technical assistance, Dr K. Fukamifor his gift of the anti-PIP₂ antibody, and J. Knight for helpin editing the manuscript.

Received for publication September 14, 1998; accepted January 12, 1999.

Literature Cited

Top
Summary
Introduction
Materials and Methods
Results
Discussion
Literature Cited

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