RGS-GAIP, a GTPase-activating Protein for Galpha i Heterotrimeric G Proteins, Is Located on Clathrin-coated Vesicles

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Vol. 9, Issue 5, 1123-1134, May 1998

RGS-GAIP, a GTPase-activating Protein for G $alpha$ _i Heterotrimeric G Proteins, Is Located on Clathrin-coated Vesicles

Luc De Vries, Eric Elenko, J. Michael McCaffery, Thierry Fischer, Laura Hubler, Tammie McQuistan, Nicki Watson, and Marilyn G. Farquhar^*

Division of Cellular and Molecular Medicine and Department of Pathology, University of California, San Diego, La Jolla, California 92093-0651

Submitted October 31, 1997; Accepted February 11, 1998
Monitoring Editor: Suzanne R. Pfeffer

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

RGS-GAIP (G $alpha$ -interacting protein) is a member of the RGS (regulator of G protein signaling) family of proteins that functionsto down-regulate G $alpha$ _i/G $alpha$ _q-linked signaling. GAIP is a GAP or guanosinetriphosphatase-activating protein that was initially discoveredby virtue of its ability to bind to the heterotrimeric G proteinG $alpha$ _i3, which is found on both the plasma membrane (PM) and Golgimembranes. Previously, we demonstrated that, in contrast to mostother GAPs, GAIP is membrane anchored and palmitoylated. In thiswork we used cell fractionation and immunocytochemistry to determinewith what particular membranes GAIP is associated. In pituitarycells we found that GAIP fractionated with intracellular membranes,not the PM; by immunogold labeling GAIP was found on clathrin-coatedbuds or vesicles (CCVs) in the Golgi region. In rat liver GAIPwas concentrated in vesicular carrier fractions; it was not foundin either Golgi- or PM-enriched fractions. By immunogold labelingit was detected on clathrin-coated pits or CCVs located near thesinusoidal PM. These results suggest that GAIP may be associatedwith both TGN-derived and PM-derived CCVs. GAIP represents thefirst GAP found on CCVs or any other intracellular membranes.The presence of GAIP on CCVs suggests a model whereby a GAP isseparated in space from its target G protein with the two cominginto contact at the time of vesicle fusion.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Classical G protein-mediated signaling pathways are three-component systems consisting of serpentine (seven-transmembranedomain) plasma membrane (PM) receptors, heterotrimeric G proteinscomposed of $alpha$ , $beta$ , and $gamma$ subunits, and an effector, usually anenzyme or an ion channel (Gilman, 1987; Bourne et al., 1990; Neer,1995; Hamm and Gilchrist, 1996). The newly discovered family ofproteins known as RGS proteins (regulators of G protein signaling)constitute a fourth component of these systems (Dohlman and Thorner,1997; Koelle, 1997; Neer, 1997; Berman and Gilman, 1998). RGSproteins serve as guanosine triphosphatase-activating proteins(GAPs) that accelerate the guanosine triphosphatase activity ofG $alpha$ i/G $alpha$ q subunits by stabilizing the G $alpha$ subunit in its guanosinetriphosphate (GTP)-to-guanosine diphosphate (GDP) transition state(Berman et al., 1996), returning them to their inactive GDP-boundform (Berman et al., 1996; Hunt et al., 1996; Watson et al., 1996),and thereby terminating the G protein signal. The RGS proteinfamily has been implicated in desensitization and negative regulationof heterotrimeric G protein-signaling pathways in yeast, fungi,and nematodes (Dohlman et al., 1996; Koelle and Horvitz, 1996;Yu et al., 1996). In mammalian cells, RGS proteins have been implicatedin the negative regulation of MAP kinase and phosphoinositide-phospholipaseC activity and a loss of inhibition of adenylate cyclase activityby G $alpha$ i subunits (Druey et al., 1996; Chatterjee et al., 1997;Huang et al., 1997; Yan et al., 1997). RGS proteins may also regulatecell death as suggested by the finding that A28-RGS14 is transcriptionallyactivated by the tumor suppressor, p53 (Buckbinder et al., 1997).The negative regulation of these cellular processes has been assumedto be due to the GAP activity of RGS proteins. However, RGS proteinfamily members also have recently been suggested to function aseffector antagonists that compete for effector binding to G $alpha$ (Hepleret al., 1997; Berman and Gilman, 1998).

GAIP (G $alpha$ interacting protein) was the first RGS protein shown to interact directly with the heterotrimeric G $alpha$ _i3 subunit throughthe RGS domain common to all family members (De Vries et al.,1995) and the first, along with RGS4, shown to have GAP activity(Berman et al., 1996). Up to now, no RGS protein has been clearlylocalized within the cell. This is an important issue becausethere are already more mammalian RGS family members (>20) thanG $alpha$ i/G $alpha$ q subunits, and multiple RGS proteins are expressed in thesame tissue or cell type (De Vries et al., 1995; Chen et al.,1996; Druey et al., 1996; Hunt et al., 1996; Chen et al., 1997;Faurobert and Hurley, 1997; Snow et al., 1997).

Heterotrimeric G proteins have been localized on intracellular membranes as well as on the PM and appear to play a role incontrol of endocytic and secretory pathways (Bomsel and Mostov,1992; Helms, 1995; Nürnberg and Ahnert-Hilger, 1996). G $alpha$ _i3 isfound on Golgi membranes (Stow et al., 1991; Wilson et al., 1994;Denker et al., 1996), and overexpression of G $alpha$ _i3 was found toslow transport of newly synthesized proteins along the exocyticpathway (Stow et al., 1991). Previously we showed that in AtT-20stably expressing GAIP, most of the GAIP (80-90%) is membraneassociated and palmitoylated most likely via its cysteine stringmotif (De Vries et al., 1996), but the nature of the membranesto which GAIP is anchored has not been established. Key unansweredquestions are whether GAIP is associated with Golgi membranesor the PM and whether it is present on the same membrane domainsas G $alpha$ _i3. Here we used cell fractionation and immunocytochemistryto determine where GAIP is located and report the unexpected findingthat GAIP is not found on either the PM or Golgi membranes butis associated with clathrin-coated buds and vesicles (CCVs).

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Materials

Male rats (100-150 g) were from Harlan Sprague Dawley (Indianapolis, IN), DMEM medium from the UCSD Cell Core Facility (LaJolla, CA), FCS from GIBCO-BRL (Gaithersburg, MD), and horse serumfrom Hyclone Laboratories (Logan, UT). Wheat germ agglutinin (WGA)-agaroseand the 5'-nucleotidase kit were purchased from Sigma Chemical(St. Louis, MO). The ECL detection kit was from Amersham LifeSciences (Arlington Heights, IL). FITC-conjugated donkey anti-rabbitF(ab')₂ and Texas Red-conjugated donkey anti-mouse F(ab')₂ cross-absorbedagainst human, mouse, rat, chicken, and goat IgG were purchasedfrom Jackson ImmunoResearch Laboratories (West Grove, PA). Goatanti-rabbit or anti-mouse IgG conjugates (5 or 10 nm gold) werepurchased from Amersham.

Antibodies

Antiserum was prepared against human GAIP_23-217, which includes the RGS domain (amino acids 80 to 206), shared withother RGS family members. Antisera were also generated againstthe N terminus and C terminus of GAIP, which are unique. GAIP_23-217was subcloned into pGEX-KG, expressed as a glutathione S-transferase(GST) fusion protein that was affinity purified on glutathioneagarose beads, and injected into rabbits. For the N-terminal-specificantiserum, a PCR fragment of human GAIP DNA (coding for residues1-79) was cloned into 5' EcoRI and 3' SalI sites of the pET28avector (Novagen, Madison, WI). His6-tagged N-terminal GAIP proteinwas produced in Escherichia coli (strain BL21(DE3)), purifiedby affinity chromatography, and injected into rabbits. For theC-terminal-specific antiserum, a peptide, QGPSQSSSEA, correspondingto the last 10 amino acids of GAIP (208-217), was coupled to keyholelimpet hemocyanin and injected into rabbits. The antiserum wasaffinity purified on the same peptide. The N-terminal antiserum,anti-GAIP (N), recognized 10 ng affinity-purified full-lengthGST-GAIP by immunoblotting at 1:4000, and the affinity-purifiedC-terminal IgG, anti-GAIP (C), detected 40 ng GST-GAIP at 1.2µg/ml. All antisera recognized a single, 25-kDa band by immunoblotting(Figure 1A) or immunoprecipitation (Figure 1B) of a lysate prepared,respectively, from unlabeled or ³⁵S-methionine-labeled AtT-20 cells stably expressing HA-GAIP (DeVries et al., 1996).

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Figure 1. Characterization of anti-GAIP antibodies demonstrating that they recognize only GAIP, a ~25 kDa protein, by immunoblotting (A) or immunoprecipitation (B) of a lysate from AtT-20 pituitary cells stably expressing HA-GAIP. (A) Cells were homogenized, centrifuged at 600 × g, and the postnuclear supernatant was solubilized in Laemmli sample buffer. The proteins (50 µg/lane) were separated by SDS-PAGE, transferred to PVDF membranes, and immunoblotted with anti-HA (1 µg/ml; lane 1); anti-GAIP (C) antiserum (1:8000; lane 2), or anti-GAIP (N) antiserum (1:4000; lane 3) followed by appropriate goat anti-mouse or anti-rabbit IgG coupled to HRP and detection by ECL. (B) Cells were labeled for 4 h in 100 µCi/ml Easytag (Dupont, Boston, MA) after which they were homogenized, and a postnuclear supernatant was prepared and solubilized in RIPA buffer. The lysate was precleared with 20 µl Protein A/G-Sepharose (mAb 16B12) or protein A-Sepharose (rabbit sera), after which GAIP was precipitated with anti-HA (5 µg/ml; lane 1), anti-GAIP (N) (lane 2), anti-GAIP (C) (lane 3), or anti-GAIP_23-217 (lane 4) antisera diluted 1:333, and the immunoprecipitates were separated by SDS-PAGE and detected by autoradiography.

MAb 16B12 against the hemagglutinin (HA) epitope was purchased from BABCO (Berkeley, CA). Polyclonal antiserum to calnexinwas a gift from J. Bergeron (McGill University, Montreal, Quebec,Canada). Mouse monoclonal antibodies against bovine and humanclathrin (heavy chain) were obtained from Polysciences (Warrington,PA) and Dr. Francis Brodsky (University of California, San Francisco,CA), respectively. Polyclonal antiserum to caveolin was purchasedfrom Transduction Laboratories (Lexington, KY). The EC polyclonalantibody against G $alpha$ _i3 was kindly provided by Dr. A. Spiegel (NIDDK,Bethesda, MD). Rabbit antiserum to $alpha$ -mannosidase II (Man II) wasprepared as described (Velasco et al., 1993).

Cell Culture

Murine AtT-20/D-16v pituitary cells, obtained from Richard Mains (Johns Hopkins University, Baltimore, MD), were grown inDME-high glucose, supplemented with 10% horse serum, 2.5% FCS,penicillin G, and streptomycin sulfate. AtT-20 cells stably expressingHA-tagged GAIP were prepared and grown as described previously(De Vries et al., 1996).

Subcellular Fractionation

AtT-20 cells were fractionated as described by Wendland and Scheller (1994). Briefly, cells of two confluent 100-mm plateswere combined by scraping into 1 ml ice-cold PBS containing PMSF(1 mM) and aprotinin (100 U/ml). All the following steps wereperformed at 4°C. The cells were homogenized by ten passages througha 30.5 gauge needle, and a postnuclear supernatant (PNS) was preparedby centrifugation for 10 min at 5000 × g. Five hundred microliterswere layered on a discontinuous sucrose gradient (0.2, 0.4, 0.6,1.0, 1.4, and 1.8 M, 750 µl each) and centrifuged for 2 h at 24,000rpm (Beckman SW50.1 rotor). Twelve fractions (400 µl) were collectedfrom the top and centrifuged for 1 h at 100,000 × g. The resultantpellets were solubilized in Laemmli sample buffer, and the proteinswere separated by SDS/PAGE. Quantitation of the amount of GAIPin cell fractions was obtained by densitometry using the ScanAnalysisprogram (Biosoft, Cambridge, United Kingdom).

Rat liver homogenization and preparation of cytosol and total microsomal membranes were as described previously (Jin et al.,1996). Briefly, total microsomal membranes were adjusted to 1.24M sucrose and loaded at the bottom of a 32-ml discontinuous sucrosegradient composed of 8 ml each of 1.18, 1.15, 0.86, and 0.25 Msucrose and centrifuged at 82,000 × g (25,000 rpm, SW28 rotor)for 3 h. Bands at the interface between 0.25 M/0.86 M and 0.86M/1.15 M sucrose, enriched in Golgi elements, were collected anddesignated Golgi light and Golgi heavy fractions (Saucan and Palade,1994). Fractions 1.15 and 1.18 were defined as carrier vesiclefraction 1 and 2 (CV1 and CV2), and fraction 1.24 was definedas the residual microsome fraction (RM) (Jin et al., 1996). Theprotein concentration of each fraction was determined by BCA assay(Pierce Chemical Co., Rockford, IL), and 50 µg of protein of eachfraction were solubilized in Laemmli sample buffer and separatedby SDS/PAGE.

SDS-PAGE and Immunoblotting

Proteins were separated on 10% or 12% SDS gels using a Bio-Rad minigel apparatus. After electrophoresis, the separated proteinswere transferred to polyvinylidinedifluoride (PVDF) membranes(Millipore, Bedford, MA). Membranes were incubated with primaryantibodies followed by secondary antibodies (anti-rabbit or anti-mouseIgG coupled to horseradish peroxidase, Bio-Rad) in 5% calf serum/PBS,0.1% Tween 20, for 1 h each, washed three times for 15 min eachbetween each incubation, and detected by ECL according to themanufacturer's instructions.

Depletion of Plasma Membranes from Subcellular Fractions by WGA-Agarose Absorption

WGA-agarose absorption was performed as described previously (Denker et al., 1996). Briefly, GAIP-containing fractions werediluted in PBS with protease inhibitors (chymostatin, leupeptin,antipain, and pepstatin A). Aliquots (1.0 ml) were incubated at4°C overnight with WGA-agarose (400 µg/ml). The bound fractionwas collected by sedimentation (1,000 × g, 5 min), and the nonboundfraction (PM-depleted membranes), was pelleted (100,000 × g, 1h) and solubilized in Laemmli sample buffer. Membrane proteinswere released from WGA-agarose by adding sample buffer, followedby boiling for 5 min, and separated by SDS/PAGE and immunoblotting.

5'-Nucleotidase Assay

GAIP-containing fractions (as detected by immunoblotting) from AtT-20 cells and rat liver were pooled, and 5'-nucleotidaseassays were performed on the pooled fractions as described bythe manufacturer. WGA-bound and nonbound fractions were preparedas described above, and the beads (bound fraction) were resuspendedin the same volume as the nonbound fraction. 5'-Nucleotidase activitywas measured on the total volume of both fractions and on non-WGA-treatedcontrols.

Immunocytochemistry

For immunofluorescence, AtT-20 cells were fixed in 2% paraformaldehyde (PFA) in 100 mM phosphate buffer, pH 7.4, for 1 h,followed by permeabilization with 0.1% Triton X-100 in PBS for10 min. Cells were then incubated 1 h at room temperature withprimary antibody, followed by a 1-h incubation in cross-absorbedFITC-conjugated donkey anti-rabbit F(ab')₂. Cells were washedand mounted in 25% PBS, 75% glycerol with 1 mg/ml p-phenylenediamine.

For immunogold or immunofluorescence labeling of cryosections, rat pituitary and liver were perfusion fixed in 8% PFA, 100mM phosphate buffer, pH 7.4 (15 min), followed by 4% PFA in phosphatebuffer (1 h). Samples were cryoprotected and frozen in liquidnitrogen as described (Hobman et al., 1992; McCaffery and Farquhar,1995). Semithin (0.5-1.0 µm) cryosections were prepared and incubatedwith primary rabbit polyclonal or mouse monoclonal antibodies(3 h at 4°C) followed by incubation in cross-absorbed FITC-conjugateddonkey anti-rabbit or TRITC-conjugated donkey anti-mouse F(ab')₂(1 h at 4°C). Ultrathin cryosections were prepared and incubated2 h at 4°C with primary antibodies in 10% FCS/PBS, followed by5- or 10-nm gold-conjugated goat anti-rabbit or anti-mouse IgG(2 h at 4°C). Grids were stained in 2% neutral uranyl acetate(10 min), adsorption-stained with 0.2% neutral uranyl acetate,0.2% methyl cellulose, and 3.2% polyvinyl alcohol, and observedin a JEOL 1200 EX-II (JEOL USA, Peabody, MA) or Philips CM-10electron microscope (Philips Electronic Instruments, Mahwah, NJ).

For quantitation, the number of gold particles/µm PM length was determined by counting the number of gold particles and tracingthe membrane contour with a cartographer's wheel. The number ofgold particles/µm membrane of coated buds and coated vesicleswas determined as follows: gold particles on coated buds or CCVswere counted in 16 fields each from pituitary and liver containinga total of 65 vesicles or buds. The diameter of the coated budsor CCVs was measured, and the mean diameter (~90 nm) and averagecircumference (2 $pi$ r X 45 = 0.28 µm) were calculated. The resultswere expressed as gold particles/µm membrane.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

While the function of GAIP as a GAP and the fact that it is anchored to membranes have been established, its localizationin the cell has not been determined. To localize endogenous GAIP,we prepared GAIP-specific antibodies against the C and N terminiof GAIP (outside the 120-amino acid RGS domain) and determinedthe distribution of GAIP by cell fractionation and by immunofluorescenceand immunogold labeling on cultured AtT-20 pituitary cells andrat liver and pituitary tissue because they express high levelsof endogenous GAIP (De Vries et al., 1995).

GAIP Fractionates with Intracellular Membranes in Pituitary Cells

Initially we prepared mouse pituitary AtT-20 cell fractions on sucrose density gradients using a procedure designed to separatelight membranes (PM, Golgi, and other smooth membranes) from heavymembranes (ER, dense-core vesicles, and secretory granules) (Wendlandand Scheller, 1994). When the fractions were solubilized and immunoblottedfor marker proteins, calnexin, a resident ER protein (Wada etal., 1991), sedimented with heavy fractions and peaked in fractions10-12, whereas the Golgi marker Man II (Velasco et al., 1993)was found only in light fractions (1-3) (Figure 2). GAIP was foundin fractions 3-7 of intermediate density (Figure 2), whereas G $alpha$ _i3codistributed with Man II in light fractions (1-3). Thus the distributionof GAIP and G $alpha$ _i3 overlapped only in fraction 3, which contained14% of the total GAIP in the gradient, with the remainder (86%)found in fractions 4-7. To eliminate the possibility that thepresence of GAIP was due to contaminating PM, we treated fractions3-7 with WGA-Agarose to selectively remove PM (Denker et al.,1996). As anticipated, WGA-bound fractions were enriched in thePM marker 5'-nucleotidase (Figure 3A) (Drummond and Masanobu,1971); however, GAIP remained in the nonbound fraction and wasnot detected in the bound fraction (Figure 3B). These resultsindicate that, in AtT-20 pituitary cells, GAIP is associated withintracellular membranes, not the PM, and has a distinct distributionfrom ER, Golgi, or PM markers.

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Figure 2. Distribution of GAIP in AtT-20 cell fractions prepared by sucrose density centrifugation as described in MATERIALS AND METHODS. The ER marker calnexin peaks in heavy fractions with the majority (71%) in fractions 9-12. The Golgi marker Man II and G $alpha$ _i3 are found in light fractions 1-3, which also contain PM. Fractions 1-3 contain 15, 44, and 40%, respectively, of the total G $alpha$ _i3 in the gradient. GAIP is associated with fractions 3-7 of intermediate density, which have 14, 17, 38, 17, and 13%, respectively, of the total. Thus, the overlap between the distribution of GAIP and that of G $alpha$ _i3 is limited to fraction 3 and is minimal (14%). Fractions were lysed in Laemmli buffer, and proteins from each fraction were separated by SDS-PAGE, transferred onto PVDF membranes, reacted with anti-GAIP (C) antiserum (diluted 1:2000) followed by goat anti-rabbit IgG coupled to HRP (1:3000), and immunoreactivity was detected by chemiluminescence (ECL).

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Figure 3. GAIP is associated with intracellular membranes in pituitary cells. GAIP-containing fractions 3-7 prepared from AtT-20 cells (see Figure 2) were pooled and diluted in PBS with protease inhibitors (chymostatin, leupeptin, antipain, and pepstatin A), and 1.0-ml aliquots were incubated at 4 C overnight with WGA-agarose (400 µg/ml) to deplete them of PM. Bound (B) and nonbound (NB) membranes were assayed for 5'-nucleotidase activity (upper panel) and solubilized and immunoblotted for GAIP (lower panel). Most (80%) of the 5'-nucleotidase activity is found in the bound fraction. GAIP is found in the nonbound fraction. Data are means ± SD of three independent experiments.

GAIP Is Localized on Clathrin-coated Buds or Vesicles Located Near the TGN in Pituitary Cells

When GAIP was localized by immunofluorescence in AtT-20 cells (Figure 4A) and semithin cryosections of rat pituitary (Figure4B), punctate staining for GAIP was distributed throughout thecytoplasm but was concentrated in the Golgi region. The punctatepattern was most evident in semithin cryosections (arrow, Figure4B). No PM staining was observed.

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Figure 4. GAIP is concentrated in the Golgi region (arrows) in AtT-20 pituitary cells (A) and in rat pituitary tissue (B). No staining of the plasma membrane is seen. AtT-20 cells or semithin cryosections of rat pituitary tissue were fixed in 2% paraformaldehyde in 100 mM phosphate buffer, incubated with affinity-purified, anti-GAIP (C) IgG followed by donkey anti-rabbit F(ab')₂-Texas Red, and examined by immunofluorescence. n, Nucleus. Scale bars, 10 µm.

To determine the nature of the compartment in which GAIP is located, we carried out immunogold labeling at the EM level onultrathin cryosections of rat pituitary. We detected GAIP on coatedvesicles, 70-100 nm diameter, located mainly on the trans sideof the Golgi stack (Figure 5, A and B, and Figure 6A) or on coatedbuds in continuity with tubular cisternae (Figure 6,B-D). Whensections were double labeled for clathrin, the major coat proteinof CCVs (Brodsky, 1997; Robinson, 1997), clathrin, and GAIP werelocalized on the same vesicles (Figure 5, C-G). No staining ofthe PM was evident (Figure 6A).

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Figure 5. GAIP is found on CCVs located in the Golgi region of rat pituitary cells by immunoelectron microscopy. (A-B) Ultrathin cryosections of pituitary sections labeled with affinity-purified anti-GAIP (C) IgG detected with 5 nm gold. GAIP is localized predominantly on the outer (cytoplasmic) surface of coated buds (arrowheads) or vesicles (arrows) found on the trans side (trans) of the Golgi cisternae (Gc) in a somatotrope (growth hormone-producing cell). Only rarely is GAIP seen on tubular elements with buds (asterisk), which usually are not labeled. Secretory granules (sg), also concentrated on the trans side of the stack, are found in the vicinity of the labeled vesicles. (C-G) Similar preparations of sections double labeled for GAIP (5 nm gold) and clathrin (10 nm gold) showing their presence on the same vesicles. Rat pituitary was fixed in 8% paraformaldehyde (PFA), 100 µM phosphate buffer, pH 7.4 (15 min), followed by 4% PFA in phosphate buffer (1 h), and ultrathin cryosections were incubated as described in MATERIALS AND METHODS. Scale bars, 0.1 µm.

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Figure 6. GAIP is present on clathrin-coated buds (arrowheads) and CCVs (arrows) but is not detected on the PM (pm) or tubular cisternae with coated buds. (A) Numerous coated buds located in the Golgi region are heavily labeled for GAIP. Counts of gold particles indicate that labeling of buds is ~90× higher than that on the tubular cisternae with which they are in continuity. The plasma membrane (pm) and Golgi membranes (Gc) are not labeled above background. (B-D) Enlargement of tubular cisternae with coated buds heavily labeled for GAIP. Note the lack of labeling of the tubular cisternae with which the buds are in continuity. Preparation same as Figure 5. Scale bars, 0.1 µm.

The abundant GAIP labeling of coated buds contrasted markedly with the sparse labeling of the membranes of the tubular cisternaewith which they were in continuity. Counts of gold particles/µmmembrane revealed that the concentration of gold particles oncoated buds and vesicles (10.4 gold particles/vesicle or 37/µmmembrane) was 93× that of the membranes of the tubular cisternaewith which they were in continuity (0.4/µm membrane). We concludethat GAIP is concentrated on clathrin-coated buds and CCVs locatedon the trans side of the Golgi stack in rat pituitary cells.

GAIP Is Concentrated in Vesicular Carrier-enriched Fractions from Rat Liver

Next we determined the distribution of GAIP in rat liver $---$ a well characterized system in which fractions enriched in carriervesicles can be separated from Golgi and other membranes by sucrosegradient centrifugation (Saucan and Palade, 1994; Jin et al.,1996). Golgi light (GL), Golgi heavy (GH), carrier vesicle 1 and2 (CV1 and CV2), and RM fractions were prepared, solubilized,and immunoblotted for GAIP and marker proteins. GAIP was mostabundant in CV1, CV2, and RM fractions, with the peak in CV2 (Figure7). No GAIP signal was detected under these conditions in theGL fraction, and only trace amounts of GAIP were found in theGH fraction. Densitometric analysis established that GAIP is 18×more abundant in CV1 and 26× more abundant in CV2 than in GH.CV1 and CV2 fractions typically contain a mixture of transcytoticvesicles, vesicles derived from early and late endosomes, TGN-derivedvesicles, and ER-to-Golgi transport vesicles (Saucan and Palade,1994; Jin et al., 1996). G $alpha$ _i3 showed a much broader distributionacross the gradient than GAIP (Figure 7) but was most abundantin the GH and CV1 fractions. The Golgi marker Man II was foundmainly in the Golgi fractions (GL and GH) as expected (Figure7). Interestingly, GAIP did not cofractionate with caveolin (Figure7), a protein said to be associated with G protein-signaling complexes(Li et al., 1995). To prove that the GAIP signal was not due toPM contamination of the CV1, CV2, and RM fractions, we pooledthese fractions and treated them with WGA-agarose to remove PM.We obtained similar results as with AtT-20 cells: the PM marker5'-nucleotidase was highly enriched in the WGA-bound fraction(Figure 8A), but GAIP was found exclusively in the nonbound fraction(Figure 8B). From these results we conclude that 1) GAIP is associatedwith intracellular membranes rather than the PM in rat liver;and 2) GAIP is most abundant in fractions enriched in transportvesicles.

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Figure 7. Distribution of GAIP in fractions prepared from rat liver. GAIP is concentrated in fractions enriched in carrier vesicles (CV1 and CV2). It is not detected in Golgi light (GL) fractions and is barely detectable in Golgi heavy (GH) fractions. Rat liver was homogenized and fractions were prepared by sucrose gradient centrigugation as described in MATERIALS AND METHODS. Fifty micrograms each of Golgi light (GL), Golgi heavy (GH), carrier vesicles 1 and 2 (CV1 and CV2), and residual microsome (RM) fractions were solubilized in Laemmli buffer and immunoblotted for GAIP (N-terminal antibody, dilution 1:4000), G $alpha$ _i3 (EC antibody, dilution 1:1000), Man II (dilution 1:2000), and caveolin (dilution 1:4000) as in Figure 1. The presence of two bands for GAIP is likely due to posttranslational modification (palmitoylation or phosphorylation).

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Figure 8. GAIP is associated with intracellular membranes in rat liver. Fractions CV1, CV2, and RM (see Figure 7) were pooled and treated with WGA to remove PM. Bound (PM) and nonbound (intracellular membranes) fractions were assayed for 5'-nucleotidase activity (A) or solubilized and immunoblotted for GAIP (B). Most (85%) of the 5'-nucleotidase activity is found in the bound fraction (B), whereas GAIP is found only in the nonbound fraction (NB). Data are means ± SD from three independent WGA treatments.

GAIP Is Localized on Clathrin-coated Pits and Vesicles Located Near the PM in Rat Liver

To determine the nature of the transport vesicles with which GAIP is associated, we carried out immunofluorescence on semithincryosections of rat liver. With anti-GAIP antibodies, punctatestaining was seen at the periphery of hepatocytes, particularlyalong the sinusoidal domain of the PM (Figure 9B). Little or nostaining for GAIP was seen in the Golgi region. This suggestedthat GAIP is located at or near the PM. Double labeling for GAIPand clathrin showed a striking overlap in their distribution atthe cell periphery, suggesting these proteins may reside in thesame structures (Figure 9C). To determine whether this is thecase, we carried out immunogold labeling on rat liver sectionswith affinity-purified anti-GAIP (C) antibodies. We found GAIPassociated with coated vesicles located near the PM (Figure 10,A-E). Occasionally, labeling for GAIP was found on coated pitsdistributed along the sinusoidal PM (Figure 10F), suggesting GAIP'sassociation with endocytic vesicles. By contrast, the PM adjacentto the coated pits showed little staining. Counts of gold particlesindicated that GAIP is 60× more concentrated on coated buds orvesicles (7.6 gold particles/vesicle or 27/µm membrane) as onthe noncoated regions in continuity with the coated buds (0.45gold particles/µm membrane). By double immunogold labeling forGAIP and clathrin, GAIP colocalized with clathrin on the samevesicles (Figure 10, G-I). We also found variable mitochondrialstaining with anti-GAIP antibodies, an observation that is currentlyunder investigation. We conclude that in rat liver, GAIP is localizedon coated pits and CCVs, very likely of endocytic origin.

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Figure 9. GAIP is distributed near the PM in rat liver. Staining for both GAIP (B) and clathrin (C) is found at the periphery of hepatocytes concentrated along the sinusoidal domain of the PM (arrows). The corresponding phase contrast image is shown in panel A. Semithin cryosections of rat liver were fixed in 2% paraformaldehyde in 100 mM phosphate buffer, pH 7.4, for 1 h, and incubated with affinity-purified, anti-GAIP (C) IgG followed by donkey anti-rabbit F(ab')₂-Texas Red, and examined by immunofluorescence. n, Nucleus. Scale bars, 10 µm.

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Figure 10. Immunogold labeling demonstrating GAIP's association with clathrin-coated pits and vesicles located near the sinusoidal PM in rat liver. (A and B) Numerous vesicles are labeled for GAIP. Note that the PM (pm) itself with which the coated pits are sometimes in continuity is not labeled. (G-I) Double labeling for GAIP (5 nm gold) and clathrin (10 nm gold) demonstrating their presence on the same vesicles. Rat liver was fixed in 8% paraformaldehyde (PFA), 100 mM phosphate buffer, pH 7.4 (15 min), followed by 4% PFA in phosphate buffer (1 h), and incubated as in Figure 4. Scale bars, 50 nm.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

We showed previously that GAIP is anchored to membranes by palmitoylation, most likely via its cysteine string motif (De Vrieset al., 1996). Palmitoylation is a reversible lipid modificationand, in the case of G $alpha$ _i proteins, is considered to regulate theirassociation with specific subdomains of the PM (Wedegaertner etal., 1995; Mumby, 1997). Here we show that GAIP cosediments withintracellular membranes by cell fractionation and is not detectedin WGA-purified PM, indicating that GAIP is located on intracellularmembranes rather than the PM. By immunofluorescence and immunoelectronmicroscopy, we clearly established that GAIP is found on clathrin-coatedbuds and CCVs in several cell types. Two general subclasses ofCCVs are distinguished based on their origin: 1) CCVs derivedfrom the TGN involved in the transport of lysosomal enzymes andmembrane proteins to late endosomes and/or lysosomes, and 2) CCVsderived from the PM or from endosomes involved in receptor-mediatedendocytosis (Brodsky, 1997; Robinson, 1997). GAIP appears to bepresent on both general subclasses of CCVs, with the TGN-derivedCCVs predominating in pituitary cells and PM-derived CCVs predominatingin hepatocytes and several cultured cell lines (NRK, HeLa). TGN-derivedCCVs are known to carry lysosomal enzymes bound to mannose 6-phosphatereceptors destined for delivery to lysosomes via early or lateendosomes. PM (coated pit)-derived CCVs are involved in the internalizationof a number of receptors and their cargo including G protein-coupledreceptors (Zhang et al., 1996). Recently, additional less wellcharacterized populations of CCVs have been described whose functionsare unclear (Robinson, 1997). GAIP is widely expressed in manytissues (pituitary, liver, lung, placenta, heart), but its expressionis low in brain (De Vries et al., 1995), which is a rich sourceof CCVs. Whether GAIP is present on all CCVs or only on specificsubpopulations of CCVs remains to be established.

GAIP is the first GAP to be localized on CCVs. Except for ras-GAP whose putative relocation to the PM has been documented(Clark et al., 1991), all other GAPs are cytosolic proteins. GAIPis the first RGS protein to be located within the cell, and withthe exception of RGS3 and SST2, there is little information onwhether or not other family members are membrane associated. RGS3has been shown to sediment in membrane fractions (Neill et al.,1997), and Sst2, the yeast RGS, codistributes on sucrose densitygradients with PM and Golgi markers and with Gpa1, the yeast G $alpha$ subunit with which it interacts (Dohlman et al., 1996). The structureof RET-RGS, found in retina, suggests it may be a membrane proteinbecause it has a predicted transmembrane domain and a cysteinestring motif similar to that found in GAIP (Faurobert and Hurley,1997).

Our cell fractionation results indicate little overlap in the distribution of GAIP and G $alpha$ _i3 in AtT-20 pituitary cells andonly a partial overlap in rat liver. G $alpha$ _i3 has been localized toGolgi membranes and to caveolae-enriched fractions (Sargiacomoet al., 1993) but not to CCVs in the cell models and tissues previouslystudied, including rat pituitary (Wilson et al., 1994) and pancreas(Denker et al., 1996). Interestingly, it has recently been reportedthat GAIP regulates a G $alpha$ _i3-dependent autophagy pathway in intestinalcells (Ogier-Denis et al., 1997).

It is still not clear whether G $alpha$ _i3 acts through classical or alternative G protein cycles on intracellular membranes, sinceno G protein-coupled receptors, effectors, or $beta$ $gamma$ subunits havebeen detected to date on intracellular membranes (Helms, 1995).The localization of GAIP on clathrin-coated buds and CCVs suggestsa model for regulation of G $alpha$ _i3 in which GAIP and G $alpha$ _i3 are locatedon different membrane domains, and GAIP is transported via vesiculartransport to its target G $alpha$ subunit. According to this model, onlyupon fusion of the vesicle with its target would the GAIP on vesiclesand the G $alpha$ subunit on membranes come into transient contact. Alternatively,GAIP might function to turn off G protein signaling during budding.However, its presence on CCVs suggests GAIP's involvement in downstreamevents. In either model the possibility should be considered thatGAIP could act, not only as a GAP to turn off G protein signaling,but also as an effector antagonist (Berman and Gilman, 1998).Spatial separation may provide an additional layer of regulationto assure that the GAP and its target are only transiently broughtinto contact via vesicular transport when a particular signaltransduction cascade is activated.

Our work raises several intriguing questions: 1) How is GAIP targeted to CCVs, i.e., are there specific targeting signalsencoded in its sequence? Or, does GAIP's interaction with otherproteins determine its localization? 2) Are other RGS proteinsfound on transport vesicles or do they have compartment-specificor domain-specific localizations? 3) What purpose does the concentrationof GAIP on CCVs serve?

Our findings suggest that the cell has evolved a system for regulation of intracellular G protein signaling that keeps theinactivators (GAPs) separated from the activators (G proteins).Thus, GAIP's localization on CCVs suggests a new paradigm forG protein signaling during vesicular transport.

	ACKNOWLEDGMENTS

We thank Beverly Wendland for advice on AtT-20 cell fractionation, Mingjie Jin and Lucian Saucan for advice on fractionationof rat liver, and Sheryl Denker for useful discussions on WGAtreatments. This work was supported by NIH grants CA-58689 andDK-17780 to M.G.F. E.E. was supported by NIH training grant 5T32 CA-67754, L.H. by fellowship CA-66289 from the National CancerInstitute, and T.F. by fellowships from the Foundation pour laRecherche Medicale and the Association pour la Recherche sur leCancer.

	FOOTNOTES

^* Corresponding Author.

Abbreviations used: CCVs, clathrin-coated vesicles; GAIP, G $alpha$ interacting protein; HA, hemagglutinin; PFA, paraformaldehyde;PM, plasma membrane; PNS, postnuclear supernatant; PVDF, polyvinylidinedifluoride;RGS, regulator of G protein signaling; RM, residual microsomes.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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