Rab2 Protein Enhances Coatomer Recruitment to Pre-Golgi Intermediates*

Ellen J. TisdaleDagger § and Michael R. Jackson

From the Dagger  Department of Pharmacology, Wayne State University School of Medicine, Detroit, Michigan 48201 and the R. W. Johnson Pharmaceutical Research Institute, San Diego, California 92121

    ABSTRACT
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Abstract
Introduction
Procedures
Results
Discussion
References

The Rab2 protein is a resident of pre-Golgi intermediates and required for vesicular transport in the early secretory pathway. We have previously shown that a peptide corresponding to the amino terminus of Rab2 (residues 2-14) arrests protein traffic prior to a rate-limiting event in VSV-G movement through pre-Golgi structures (Tisdale, E. J., and Balch, W. E. (1996) J. Biol. Chem. 271, 29372-29379). To determine the mechanism by which this peptide inhibits transport, we investigated the effect of the Rab2 peptide on the distribution of the beta -COP subunit of coatomer because COPI partially localizes to pre-Golgi intermediates. We found that the peptide caused a dramatic change in the distribution of pre-Golgi intermediates containing beta -COP. A quantitative binding assay was employed to measure recruitment of beta -COP to membrane when incubated with the Rab2 (13-mer). Peptide-treated microsomes showed a 25-70% increase in the level of membrane-associated beta -COP. The enhanced recruitment of coatomer to membrane was specific to the Rab2 (13-mer) and required guanosine 5'-3-O-(thio)triphosphate, ADP ribosylation factor, and protein kinase C-like activity. The ability to enhance beta -COP membrane binding was not limited to the peptide. Similarly, the addition of recombinant Rab2 protein to the assay promoted beta -COP membrane association. Our results suggest that the Rab2 peptide causes the persistent recruitment of COPI to pre-Golgi intermediates which ultimately arrests protein transport due to the inability of membranes to uncoat.

    INTRODUCTION
Top
Abstract
Introduction
Procedures
Results
Discussion
References

Membrane traffic in the early secretory pathway requires the Rab1 and Rab2 GTPases (1, 2). The Rab1 protein is found in the endoplasmic reticulum (ER),1 pre-Golgi intermediates, and early compartments of the Golgi complex (3), whereas Rab2 has been immunolocalized only to pre-Golgi intermediates (4). These transport intermediates composed of vesicles and tubular clusters (VTCs) (5) are distinct from the ER and the Golgi complex (6). VTCs are morphologically defined by the proteins ERGIC-53/gp58 (p53/gp58) (7, 8) and Rab2 (4), and are the major peripheral site for COPI recruitment (9, 10).

Pre-Golgi intermediates (VTCs) sort and recycle resident proteins from itinerant proteins destined for secretion (10-12). Although the mechanism of protein recycling is unknown, it is likely to involve the COPI coat complex (coatomer and ARF) (10, 13, 14). Coatomer is a heptameric, soluble complex composed of alpha , beta , beta ', gamma , delta , epsilon , and zeta  subunits (15). Perhaps the best characterized component of coatomer is the beta -COP subunit that was first identified as an 110-kDa peripheral membrane protein associated with pre-Golgi intermediates and the cis Golgi stack (16, 17). The coat complex is recruited en bloc (18) or as a subset (19, 20) to membrane after activation of the small GTPase ADP ribosylation factor (ARF) (21, 22) and phospholipase D. Phospholipase D hydrolyzes phosphatidylcholine to phosphatidic acid which in tandem with phosphatidylinositol 4,5-bisphosphate enhances coatomer membrane association (23, 24). The binding of COP1 deforms the membrane which leads to bud formation and eventual release of a coated vesicle.

We have reported that a peptide which corresponds to residues 2-14 of Rab2 arrests protein transport by preventing the flow of cargo through pre-Golgi intermediates (VTCs) (2). The ability of this peptide to block transport in a rapid and specific manner makes it a valuable tool to dissect events in the early secretory pathway. In this study, we took advantage of the irreversible property of the peptide to determine the mechanism by which the Rab2 (13-mer) arrests transport. Our previous observation that peptide affects transport from pre-Golgi structures prompted us to look at the distribution of transport-related proteins which co-localize to VTCs. We initially analyzed the distribution of COPI by focusing on the beta -COP subunit. To our surprise, we found that the peptide had a striking affect on beta -COP recruitment. Membranes incubated with peptide showed a 25-70% increase in beta -COP binding compared with control. This increase in coatomer binding was specific to the Rab2 (13-mer) and required ARF, GTPgamma S, and protein kinase C (PKC) or a PKC-like protein. Similar results were obtained after addition of recombinant Rab2 protein to the binding assay. We propose that this enhanced COPI recruitment results in the inability of vesicles derived from pre-Golgi structures to uncoat which ultimately leads to the coupled arrest of anterograde and retrograde traffic. These data suggest that Rab2 plays a role in protein sorting and recycling from pre-Golgi intermediates.

    EXPERIMENTAL PROCEDURES
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Abstract
Introduction
Procedures
Results
Discussion
References

Materials-- Polyclonal antiserum made to peptides corresponding to beta -COP (EAGELKPEEEITVGPVQK), N-alpha -COP (yeast sequence KMLTKFESKSTRAKGYC), N-beta '-COP (PLRLDIKRKLTARSDYC), and N-epsilon -COP (APPAPGPASGGSGEVYC) were generously provided by Dr. Rohan Teasdale (R. W. Johnson Pharmaceutical Research Institute, La Jolla, CA). The serum was applied to cyanogen bromide-activated Sepharose 4B to which the immunizing peptide was coupled for affinity purification. The column was washed with 5 bed volumes of PBS and eluted with 0.1 M glycine, pH 2.8. The eluate was neutralized to pH 7.2, dialyzed against PBS, then concentrated. Peptides were synthesized at the R. W. Johnson Pharmaceutical Research Institute Protein Facility (La Jolla, CA). The monoclonal antibody to ARF (1D9) and ARF1 cDNA was a gift from Dr. Richard Kahn (Emory University, Atlanta, GA). Purified coatomer was kindly provided by Dr. M. Gerard Waters (Princeton University, Princeton, NJ). Polyclonal antiserum to Rab2 was purchased from Santa Cruz Biotechnology. Rab2 cDNA was acquired from Dr. Marino Zerial (EMBL, Heidelberg, Germany). The polyclonal serum to p58 was obtained from Dr. Jaakko Saraste (University of Bergen, Bergen, Norway). Calphostin C was purchased from Calbiochem (San Diego, CA). Chelerythrine chloride was obtained from LC Laboratories. Digotonin was acquired from Boehringer Mannheim. HRP-conjugated antibody was purchased from Bio-Rad. Monoclonal antibody to beta -COP (M3A5) and all other reagents were purchased from Sigma.

Membrane Binding Reaction-- HeLa cells were washed three times with ice-cold phosphate-buffered saline (PBS). The cells were scraped off the dish with a rubber policeman into 10 mM Hepes, pH 7.2, and 250 mM mannitol, then broken with 15 passes of a 27-gauge syringe. The broken cells were pelleted at 500 × g for 10 min at 4 °C, and the supernatant re-centrifuged at 20,000 × g for 20 min at 4 °C. The pellet containing ER, pre-Golgi, and Golgi membranes was washed with 1 M KCl in 10 mM Hepes, pH 7.2, for 15 min on ice, then centrifuged at 20,000 × g for 20 min at 4 °C. The membranes were resuspended in 10 mM Hepes, pH 7.2, and 250 mM mannitol and employed in the binding reaction as described previously (10, 14). Membranes (30 µg of total protein) were added to a reaction mixture which contained 27.5 mM Hepes, pH 7.2, 2.75 mM MgOAc, 65 mM KOAc, 5 mM EGTA, 1.8 mM CaCl2, 1 mM ATP, 5 mM creatine phosphate, and 0.2 units of rabbit muscle creatine kinase. Peptide or Rab2 protein were added to obtain the final concentration as indicated under "Results" and the reaction mixture incubated on ice for 30 min. Rat liver cytosol (50 µg) and 2.0 µM GTPgamma S were then added and the reactions shifted to 37 °C and incubated for 10 min. The binding reaction was terminated by transferring the samples to ice and then centrifuged at 20,000 × g for 10 min at 4 °C. The pellet was resuspended in sample buffer, separated by SDS-PAGE and transferred to nitrocellulose in 25 mM Tris, pH 8.3, 192 mM glycine, 20% methanol. The membrane was blocked in Tris-buffered saline (TBS) which contained 5% nonfat dry milk and 0.5% Tween 20, incubated with an affinity purified polyclonal antibody made to the EAGE peptide of beta -COP (25) or a polyclonal antibody to Rab2, or a monoclonal antibody to ARF (1D9) (26), washed, further incubated with a horseradish peroxidase (HRP)-conjugated anti-rabbit or anti-mouse antibody, developed with enhanced chemiluminescence (ECL) (Amersham), then quantitated by densitometry.

Indirect Immunofluorescence-- NRK cells plated on coverslips were permeabilized with digitonin (20 µg/ml) as outlined previously (3). Coverslips with permeabilized cells were inverted and placed in tissue culture wells that contained the transport mixture described above, preincubated on ice for 15 min with or without peptide or Rab2 protein and then incubated for 80 min at 15 °C. To terminate transport, the cells were transferred to ice and fixed in 3% formaldehyde/PBS for 10 min. Intracellular beta -COP was detected by re-permeabilization of the fixed cells with 0.05% saponin in PBS/normal goat serum for 10 min, washed with PBS, then co-incubated for 30 min with a monoclonal antibody to beta -COP (M3A5) and a polyclonal serum to p58, or with polyclonal serum to Rab2. Cells were then washed with PBS, co-stained for 30 min with Texas Red anti-rabbit antibody and fluorescein isothiocyanate anti-mouse antibody, washed, mounted, then viewed under a Zeiss Axiovert fluorescence microscope.

Purification of Recombinant Rab2 Protein and in Vitro Prenylation-- Rab2Delta 14 was generated by polymerase chain reaction using a 5'-oligonucleotide primer which introduced a start codon at the deletion site. The cDNA for Rab2 wild type and Rab2Delta 14 were cloned into pET3A (Novagen, Milwaukee, WI) and introduced into BL21 (DE3) pLysS (Novagen). A 1-liter culture was grown to an OD600 of 0.4-0.5 and induced with 0.4 mM isopropyl-beta -thiogalactopyranoside for 3 h at 37 °C. The cells were centrifuged at 5000 × g for 10 min at 4 °C, and the cell pellet resuspended in 50 mM Tris, pH 7.4, 1 mM dithiothreitol, 0.1 mM phenylmethylsulfonyl fluoride, 0.1 mM benzamidine, 1 mM EDTA, and 1% Triton X-100, then homogenized by 20 passes with a Dounce tissue grinder. Lysozyme (400 µg/ml), DNase I (40 µg/ml), and 25 mM MgCl2 were added to the homogenate and allowed to digest for 30 min at 4 °C, then centrifuged at 22,000 × g for 30 min at 4 °C. The supernatant was applied to a 70-ml column containing Q Sepharose Fast Flow (Pharmacia) equilibrated with Buffer A (50 mM Tris, pH 7.4, 10 mM MgCl2, and 1.0 mM EDTA), washed with 2 bed volumes of Buffer A, then eluted with a linear NaCl gradient (0-400 mM) in Buffer A. Three-ml fractions were collected and an aliquot of each fraction separated by SDS-PAGE and immunoblotted with a Rab2 polyclonal antibody. Rab2-enriched fractions were pooled, concentrated, and applied to a 200-ml column containing Sephacryl S-100 (Pharmacia) and eluted with Buffer A. Fractions containing Rab2 or Rab2Delta 14 proteins were identified by SDS-PAGE and immunoblotting, then pooled, concentrated, and prenylated in an in vitro reaction. Briefly, the isoprenylation reaction was performed in a total volume of 50 µl that contained 5 µg of recombinant Rab2 protein, 10 µg of geranylgeranyl pyrophosphate (Sigma), 1 mM dithiothreitol, 25 µl of rat liver cytosol, 10 mM MgCl2, 1 mM ATP, 5 mM creatine phosphate, and 0.2 units of rabbit muscle creatine kinase. The reaction was incubated for 1 h at 37 °C and then desalted through a 1-ml column of Sephadex G-25 (Pharmacia) and concentrated. The protein concentration was determined by Micro BCA Protein Assay Reagent (Pierce).

Purification of Recombinant ARF and Preparation of ARF-depleted Cytosol-- Recombinant myristoylated ARF was prepared from the BL21 bacterial strain that had been co-transformed with a plasmid encoding N-myristoyltransferase and wild type ARF1 (27). The transformed cells were induced with 1.0 mM isopropyl-beta -thiogalactopyranoside for 3 h at 25 °C in the presence of 50 µM myristate. The cells were lysed and the expressed ARF1 purified on a DEAE-Sephacel and AcA54 Ultrogel columns as described by Weiss et al. (28). For ARF depletion, rat liver cytosol was fractionation on a Superose 6 column equilibrated in 25 mM Hepes, pH 7.2, 125 mM KOAc, 2.5 mM MgOAc, and 1 mM dithiothreitol (28). ARF-enriched and ARF-depleted fractions were identified by Western blotting. Those fractions lacking ARF were pooled, and concentrated to the original volume.

    RESULTS
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Abstract
Introduction
Procedures
Results
Discussion
References

N-terminal Peptide to Rab2 Alters beta -COP Distribution-- We analyzed the distribution of beta -COP in permeabilized NRK cells incubated with or without peptide for 80 min at 15 °C by indirect immunofluorescence. Cells were incubated at this reduced temperature to accumulate and enhance visualization of pre-Golgi intermediates (VTCs). In control cells, anti-beta -COP antibody labeled the juxtanuclear Golgi complex and vesicular structures scattered throughout the cytoplasm and in proximity to the Golgi complex (Fig. 1A). This distribution of beta -COP is in agreement with that found in other cell types (6, 9, 10). In contrast, cells incubated in the presence of the Rab2 peptide displayed prominent beta -COP-labeled structures that ringed the nucleus in a collar-like manner (Fig. 1B). These cells did not appear to contain peripherally-located beta -COP-labeled vesicles. The beta -COP containing ring-like structure partially overlapped with VTCs located near the cis Golgi region that stained with the antibody to p58 (29) (Fig. 1D) and with antibody to Rab2 (Fig. 1H). Both of these polypeptides are considered marker proteins for VTCs (4, 7, 8). As we observed with antibody to beta -COP, p58 (Fig. 1D) and Rab2 (Fig. 1H)-labeled vesicles were not found in peripheral locations. In control cells, p58 (Fig. 1C) and Rab2 (Fig. 1G) were localized in vesicular elements that were concentrated in the Golgi region and dispersed throughout the cytoplasm. This staining pattern is similar to that observed with antibody to beta -COP. This striking change in VTC distribution prompted us to further explore the relationship of Rab2 to COPI recruitment.


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Fig. 1.   Rab2 (13-mer) causes redistribution of beta -COP-labeled structures. NRK cells grown on coverslips were permeabilized with digotonin, and then incubated in a complete transport mixture in the absence (A, C, E, and G) or presence (B, D, F, and H) of 50 µM Rab2 peptide for 80 min at 15 °C. The distribution of beta -COP (A and B) and p58 (C and D), or beta -COP (E and F) and Rab2 (G and H) was determined by indirect immunofluorescence as described under "Experimental Procedures." In control cells, antibody to beta -COP labeled the Golgi region and peripherally located pre-Golgi intermediates or VTCs. These structures overlap with vesicles that stain with antibody to p58 (panel C) and with antibody to Rab2 (panel G). Peptide-treated cells displayed punctate beta -COP-labeled vesicles that ringed the nucleus. This ring-like structure co-distributed with vesicles that stained with antibody to p58 (panel D) and with antibody to Rab2 (panel H).

Rab2 (13-mer) Increases Membrane-associated beta -COP-- A quantitative binding assay was used to measure beta -COP recruitment to membranes in the presence of the Rab2 peptide (10, 21). For this assay, microsomes were prepared from whole cell homogenates and washed with 1 M KCl to remove pre-bound COPI. These membranes were preincubated in buffer for 30 min on ice with or without peptide, and then supplemented with GTPgamma S and rat liver cytosol and incubated at 37 °C for 10 min. The peptide concentrations employed in the binding assay were equivalent to those which inhibit protein traffic in an in vitro transport assay (2). To terminate the reaction, membranes were collected by centrifugation, separated by SDS-PAGE, transferred to nitrocellulose, then probed with an affinity purified antibody to beta -COP. We observed in peptide-treated membranes a marked increase in beta -COP recruitment that occurred in a dose dependent manner and required GTPgamma S (Fig. 2). The amount of membrane-associated beta -COP increased ~50% when incubated with 25 µM peptide. In our previous studies (2), this peptide concentration reduced ER to Golgi transport by 50% in an in vitro transport assay. To learn if recruitment was specific to the Rab2 (13-mer), peptides were synthesized to the amino terminus of other Rab proteins and evaluated in the binding assay (see Table I). Stimulation of beta -COP membrane binding was specific to the Rab2 (13-mer). As shown in Fig. 3, a randomized form of Rab2 (13-mer) had no effect on beta -COP binding even at a concentration that results in maximum recruitment by the wild-type peptide. Likewise, a peptide that corresponds to the first 7 amino acids of Rab2 had no influence on beta -COP membrane binding. The amount of membrane-associated beta -COP was not affected by control peptides made to the analogous N-terminal domains of Rab5 and Rab3A. We also noted that a peptide to the amino terminus of Rab1B, a protein essential for ER to Golgi transport failed to recruit coatomer above the control level. These results show that the enhanced recruitment of beta -COP to membrane was specific to the Rab2 (13-mer).


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Fig. 2.   Rab2 peptide stimulates beta -COP membrane recruitment. Microsomes were prepared from HeLa cell homogenates as described under "Experimental Procedures," then preincubated with or without increasing concentrations of the Rab2 peptide for 30 min on ice. Cytosol and GTPgamma S were added to one set of membranes (closed bar), whereas the other set received only cytosol (striped bar) and then all membranes incubated for 10 min at 37 °C to promote COPI binding. Microsomes were collected by centrifugation, separated by SDS-PAGE, and immunoblotted with affinity-purified antibody to beta -COP. Rab2 peptide treatment resulted in a marked increase in membrane-associated beta -COP that required GTPgamma S.

                              
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Table I
Peptides tested in membrane binding assay
Membrane binding assay was performed as described under "Experimental Procedures."


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Fig. 3.   Enhanced beta -COP membrane binding is specific to the Rab2 (13-mer). Microsomes were prepared from HeLa cell homogenates as described under "Experimental Procedures," and then preincubated for 30 min on ice in 50 µM peptide corresponding to the amino terminus of the peptides indicated (see Table I). Cytosol and GTPgamma S were added and the membranes incubated for 10 min at 37 °C. Membranes were pelleted and then subjected to SDS-PAGE and Western blotting. The blot was incubated with a polyclonal antibody to beta -COP, then further incubated with HRP-conjugated secondary antibody and developed with ECL. The amount of recruited beta -COP was quantitated by densitometry.

The availability of affinity-purified antibodies that recognize the alpha , beta ', and epsilon  subunits of coatomer allowed us to test for co-recruitment after peptide treatment. In all cases, we observed a linear increase in membrane binding of these subunits comparable to beta -COP (data not shown). It appears that the peptide stimulates, at the very least, recruitment of a subcomplex if not all coatomer subunits.

The Rab2 Peptide Increases the Rate of beta -COP Recruitment-- We performed a time course in which membrane was incubated with or without peptide to determine whether the Rab2 (13-mer) affects the rate of coatomer recruitment to membrane. As shown in Fig. 4A, the Rab2 peptide accelerated coatomer binding that resulted in a t1/2 of ~5 min compared to t1/2 of ~7.5 min for the control. No increase in beta -COP recruitment was observed after ~10 min of incubation for both control and peptide-treated membranes. The apparent saturability was not due to the rate of COPI binding, since longer incubations times did not result in an increased level of membrane-bound beta -COP (data not shown). To further learn if the membranes were saturated with beta -COP or if cytosol was limiting, microsomes were preincubated with or without the Rab2 peptide and then GTPgamma S and increasing amounts of cytosol added. Fig. 4B shows that control and peptide-treated membranes were saturated with beta -COP when incubated with 0.1 mg of cytosol (total protein). Incubation of membranes with higher cytosol concentrations did not result in additional beta -COP recruitment. Peptide-treated membranes showed an ~ 30% increase in membrane-bound beta -COP compared with control membrane. These combined results suggest that the Rab2 (13-mer) not only affects the extent of beta -COP recruitment but also causes a rapid recruitment of COPI to membrane.


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Fig. 4.   The Rab2 peptide accelerates the rate of beta -COP recruitment to membrane. Panel A, HeLa cell membranes were incubated for increasing time in the absence (closed circle) or presence (open square) of 50 µM Rab2 peptide. At the time indicated, membranes were shifted to ice, pelleted, separated by SDS-PAGE, and transferred to nitrocellulose. The blot was probed with antibody to beta -COP and the amount of beta -COP quantitated by densitometry. Panel B, binding reactions were preincubated for 30 min at 0 °C in the absence or presence of 50 µM Rab2 peptide. Increasing amounts of cytosol and 2.0 µM GTPgamma S were then added and the reaction incubated for 20 min at 37 °C. Membranes were pelleted, subjected to SDS-PAGE and Western blotting. The amount of membrane-associated beta -COP was determined as described under "Experimental Procedures." The Rab2 peptide increased the rate and extent of beta -COP membrane binding.

Rab2 Protein Increases Membrane-associated beta -COP-- The Rab2 peptide inhibits protein traffic in an irreversible manner (2) which may result from the inability of the Rab2 protein to bind to pre-Golgi elements. We pursued this question by first establishing a dose-response curve for the Rab2 protein. The addition of 200 ng of Rab2 protein saturated the membranes (Fig. 5). The microsomal binding assay was then performed with increasing peptide concentrations in the presence of 200 ng of recombinant Rab2 protein. The amount of membrane-bound Rab2 protein did not change when co-incubated with 10-75 µM peptide (Fig. 5, inset). These results suggest that the Rab2 (13-mer) does not compete with Rab2 protein binding to membrane.


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Fig. 5.   Rab2 amino-terminal peptide does not compete with Rab2 protein membrane binding. HeLa cell microsomes were incubated with increasing concentrations of purified recombinant Rab2 protein in an assay buffer supplemented with GTPgamma S for 15 min at 37 °C. The membranes were pelleted, separated by SDS-PAGE, transferred to nitrocellulose, and the blot probed with a polyclonal antibody to Rab2. After incubation with an HRP-conjugated secondary antibody, the blot was developed with ECL and the amount of recruited Rab2 quantitated by densitometry. Membranes are saturated with 200 ng of Rab2 protein. Inset, HeLa cell membranes were preincubated with 200 ng of recombinant Rab2 protein in the presence or absence of increasing Rab2 peptide concentrations for 30 min on ice. GTPgamma S was then added and the reactions shifted to 37 °C for 15 min. Microsomes were collected by centrifugation, separated by SDS-PAGE, and immunoblotted with polyclonal antibody to Rab2, and quantitated by densitometry. The amount of membrane-bound Rab2 did not change with increasing peptide concentration which suggests that the Rab2 (13-mer) does not interfere with Rab2 protein binding to membrane.

We reasoned that if there was no competition between the peptide and the Rab2 protein for binding, then the Rab2 (13-mer) might mimic the function of the intact protein and therefore potentiate Rab2 activity. To address this possibility, the microsomal binding assay was performed by incubating membranes with three concentrations of recombinant Rab2 protein with GTPgamma S and cytosol for 15 min at 37 °C. As we observed with the Rab2 (13-mer), Rab2 protein membrane binding resulted in a dose-dependent increase in membrane-associated beta -COP (Fig. 6A). This result was further investigated in the morphological assay which showed that the Rab2 protein changed the intracellular distribution of beta -COP. In these cells we observed large beta -COP containing structures located in the perinuclear region (Fig. 7C). These structures appeared to overlap with juxtanuclear structures that labeled with antibody to p58 (Fig. 7D) and with antibody to Rab2 (Fig. 7D, inset). This accumulation of COPI containing intracellular structures in response to the Rab2 protein is consistent with the enhanced beta -COP recruitment observed in the microsomal binding assay.


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Fig. 6.   Recombinant Rab2 protein promotes beta -COP membrane association. Recombinant Rab2 wild-type protein was purified and isoprenylated in vitro, as described under "Experimental Procedures." HeLa cell microsomes were incubated with 0, 50, 100, or 200 ng of recombinant Rab2 protein (panel A) or recombinant Rab2Delta 14 protein (panel B) in assay buffer supplemented with GTPgamma S and cytosol for 15 min at 37 °C. Membranes were pelleted, separated by SDS-PAGE, transferred to nitrocellulose, and the blot probed with a monoclonal antibody to beta -COP and a polyclonal antibody to Rab2. After incubation with HRP-conjugated secondary antibodies, the blot was developed with ECL and the amount of recruited Rab2 and beta -COP was quantitated by densitometry. A co-linear increase in Rab2 and beta -COP was noted with increasing protein concentration. The amino-terminal truncated form of Rab2 had no effect on beta -COP recruitment.


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Fig. 7.   Rab2 protein alters beta -COP distribution in permealized cells. NRK cells grown on coverslips were permeabilized with digotonin, and then incubated in a complete transport mixture (panels A and B), or in a complete transport mixture supplemented with 200 ng of Rab2 protein (panels C and D) or with 200 ng of Rab2 Delta 14 (panels E and F) for 80 min at 15 °C. The distribution of beta -COP (all panels), the distribution of p58 (inset panels A, C, and E), and the distribution of Rab2 (inset panel B, D, and F) was determined by indirect immunofluorescence as described under "Experimental Procedures." In control cells, antibody to beta -COP predominantly labeled the Golgi region. Rab2 protein-treated cells displayed enhanced perinuclear beta -COP staining that overlapped with structures stained for p58 and Rab2. Arrows denote alignment of co-stained cells.

From our earlier work we know that overexpression of Rab2 wild-type caused a decrease (25%) in the processing of VSV-G to endo H-resistant forms (2). Deletion of the first 14 amino-terminal residues from Rab2 wild-type did not affect prenylation, but restored transport to control levels. To determine if a similar truncation of Rab2 wild-type could modify the ability of the protein to recruit beta -COP, we generated recombinant Rab2 Delta 14 protein and introduced the mutant protein into the binding assay. Fig. 6B shows that membranes treated with Rab2 Delta 14 did not recruit beta -COP to the level obtained by incubation with the wild-type protein. Furthermore, the truncated protein did not alter beta -COP distribution when introduced into the morphological assay (Fig. 7E). These cells displayed a similar distribution of VTCs labeled with p58 (Fig. 7F) and Rab2 (Fig. 7F, set) compared with control (Fig. 7, A and B). These combined results support our contention that the peptide functions as a bona fide domain of the Rab2 protein and more importantly, demonstrates that the amino-terminal residues of Rab2 are necessary to promote COPI binding.

ARF Enhances beta -COP Binding in Rab2 Peptide and Rab2 Protein-treated Microsomes-- Numerous studies show that the small GTPase ARF facilitates COPI binding to pre-Golgi elements and the Golgi complex (10, 21, 22). However, it has also been reported that membranes prepared from PtK1 cells can form COPI-coated vesicles in the absence of exogenous ARF (24). This ARF independent COPI recruitment requires phospholipase D activity to produce phosphatidic acid which forms stable binding sites for coatomer. On the basis of these results, we wanted to determine whether peptide recruitment of beta -COP required pre-bound ARF. Microsomes were incubated with increasing concentrations of the Rab2 (13-mer) for 10 min at 37 °C. The membranes were collected, subjected to SDS-PAGE and Western blotting, then probed with a monoclonal antibody to ARF (1D9) (26) and beta -COP. As shown in Fig. 8A, peptide stimulated a modest increase in membrane-bound ARF (see bar graph). This finding contrasts with the peptide induced linear increase of beta -COP and most likely reflects ARF-saturated membrane. In support of this interpretation, dose-response curves generated with increasing cytosol showed that the concentration used in the binding assay contains near-saturating amounts of ARF (data not shown).


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Fig. 8.   Rab2 amino-terminal peptide and Rab2 protein require ARF to stimulate beta -COP membrane binding. Panel A, HeLa cell microsomes prepared as described under "Experimental Procedures" were preincubated with increasing concentrations of the Rab2 (13-mer) for 30 min on ice. Cytosol and GTPgamma S were then added and the membranes incubated for 10 min at 37 °C. After separation by SDS-PAGE and Western blotting, the transfer was probed with antibody to beta -COP and to ARF, washed, further incubated with HRP-conjugated secondary antibody, and developed with ECL. The amount of beta -COP and ARF was quantitated by densitometry. Panel B, salt-washed microsomes were incubated with purified coatomer (75 ng) and GTPgamma S in the absence or presence of 50 µM Rab2 peptide or 100 ng of Rab2 protein for 10 min at 37 °C. To one set of binding reactions was added 75 ng of purified ARF (+). The amount of membrane-associated beta -COP was determined by densitometry. Panel C, membrane was incubated with ARF-depleted cytosol (-ARF) in the absence or presence of 100 ng of Rab2 protein or 50 µM Rab2 peptide supplemented with GTPgamma S and incubated for 10 min at 37 °C. One set of reactions was supplemented with 75 ng of ARF1 (+ARF) and incubated as above. Membranes were pelleted, separated by SDS-PAGE, transferred to nitrocellulose, and the blot probed with a monoclonal antibody to beta -COP (anti-beta -COP) and a monoclonal antibody to ARF (anti-ARF) and developed by ECL.

To further study the role of ARF in coatomer recruitment, purified components were evaluated in the binding assay. We used coatomer and ARF concentrations that were comparable to the cytosolic concentrations of these components employed in the assay. Fig. 8B shows control membranes bound a small amount of coatomer. The addition of exogenous ARF stimulated beta -COP binding. Similarly, coatomer recruitment was significantly enhanced when ARF was added to microsomes treated with the Rab2 (13-mer) or the Rab2 protein. Both Rab2 peptide- and Rab2 protein-incubated membranes recruited more beta -COP than control. As further proof for an ARF requirement in the assay, we depleted ARF from cytosol by gel filtration on a Superose 6 FPLC column (28). The binding reaction was then performed with the ARF-deficient, coatomer-containing cytosol in the presence or absence of the Rab2 (13-mer) or Rab2 protein (Fig. 8C). In these reactions, the amount of membrane-associated beta -COP was negligible. However, the addition of purified recombinant ARF to the assay restored beta -COP binding. As we observed with the purified components, the level of membrane-bound COPI is greater in reactions containing Rab2 peptide and Rab2 protein. These membranes also recruit more beta -COP than microsomes incubated with purified components suggesting that an additional cytosolic factor may promote membrane binding. Interestingly, the amount of bound ARF is comparable between control and treated membranes (Fig. 8C, anti-ARF). Most likely ARF acts catalytically to facilitate coatomer recruitment. These combined results suggest that the Rab2 peptide and protein do not "by-pass" ARF but require ARF-dependent assembly of beta -COP containing coat complex onto membrane.

Calphostin C Inhibits Rab2 Peptide and Rab2 Protein Recruitment of beta -COP-- It has been reported that ARF/coat assembly increases in response to protein kinase C (PKC) (30). We know from our previous studies that the specific PKC inhibitor calphostin C, arrests protein traffic prior to the block by the Rab2 peptide (2) and therefore PKC or a PKC-like protein functions upstream of Rab2. To determine whether PKC influenced Rab2 peptide and Rab2 protein activity, coatomer binding was assessed in the presence of calphostin C. This molecule recognizes the highly conserved cysteine-rich motif present in the PKC regulatory domain and competes for binding with diacylglycerol and phorbol esters (31, 32). Membranes preincubated with 2.5 µM calphostin C did not recruit ARF or beta -COP (Fig. 9). We observed a similar result with peptide-treated membrane. The ability of the Rab2 peptide to increase COPI binding was completely lost when membrane was co-incubated with calphostin C (Fig. 9). These membranes contained barely detectable ARF. This effect was not limited to the peptide. Membranes incubated with Rab2 protein failed to bind beta -COP when treated with calphostin C. However, calphostin C does not interfere with Rab2 protein membrane association. As we observed with the peptide, membrane-bound ARF was negligible. These data provide evidence that PKC or a PKC-like protein is an upstream effector and required for the Rab2 (13-mer) and the Rab2 protein to stimulate COPI recruitment.


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Fig. 9.   Calphostin C blocks the ability of the Rab2 peptide and Rab2 protein to stimulate beta -COP recruitment. Microsomes prepared as described under "Experimental Procedures" were preincubated with or without 2.5 µM calphostin C in the presence of 50 µM Rab2 (13-mer) or 100 ng of recombinant Rab2 protein for 30 min on ice. The membranes were then supplemented with cytosol and GTPgamma S and incubated at 37 °C for 10 min. The amount of membrane-bound beta -COP and ARF was determined as described under "Experimental Procedures." Calphostin C inhibited binding of ARF and coatomer to membranes incubated with the Rab2 (13-mer) and Rab2 protein.

To further study the role of PKC in mediating Rab2 (13-mer) and Rab2 protein-activated COPI recruitment, we performed the binding reaction with chelerythrine chloride. This molecule acts on the catalytic domain of PKC and specifically inhibits PKC kinase activity (33). Fig. 10 (lane D) shows membranes treated with 2.0 µM chelerythrine chloride bound beta -COP and ARF at a level equal to control membranes supplemented with GTPgamma S (Fig. 10, lane B). The reagent is active because control kinase reactions using bovine PKC were inhibited (data not shown). We co-incubated chelerythrine chloride and the Rab2 peptide in the binding assay. The kinase inhibitor had no influence on the ability of the Rab2 peptide to stimulate COPI binding nor did the reagent affect ARF membrane association (Fig. 10, lane E). Similarly, chelerythrine chloride did not influence beta -COP or ARF binding to Rab2 protein-treated membranes (Fig. 10, lane G). These results indicate that PKC phosphorylating activity is not required.


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Fig. 10.   PKC kinase activity is not required for COPI binding. HeLa cell membranes were preincubated with the following reagents in the absence of cytosol and GTPgamma S for 30 min on ice, then cytosol and GTPgamma S were added and incubated at 37 °C for 10 min to promote coatomer (closed bar) and ARF recruitment (open bar); lane A, control membranes, no GTPgamma S; lane B, control membranes supplemented with GTPgamma S; lane C, 50 µM Rab2 peptide and GTPgamma S; lane D, 2.0 µM chelerythrine chloride and GTPgamma S; lane E, 2.0 µM chelerythrine chloride, 50 µM Rab2 peptide and GTPgamma S; lane F, 100 ng of Rab2 protein and GTPgamma S; lane G, 2.0 µM chelerythrine chloride, 100 ng of Rab2 protein, and GTPgamma S. The amount of beta -COP and ARF recruited to membrane was quantitated as described under "Experimental Procedures."

    DISCUSSION
Top
Abstract
Introduction
Procedures
Results
Discussion
References

We previously reported that a peptide corresponding to the amino terminus of Rab2 was a potent and irreversible inhibitor of ER to Golgi transport. The Rab2 peptide did not interfere with vesicle budding from the ER nor did it prevent intra-Golgi trafficking (2). These results suggested that the Rab2 (13-mer) specifically arrested transport from VTCs. Since Rab2 immunolocalizes to pre-Golgi intermediates and the Rab2 peptide interferes with traffic from these intermediates, we wished to learn if the peptide influenced other transported-related proteins which also target to these structures. Our thought was that this information might shed light on the mechanism by which the Rab2 peptide inhibits protein trafficking. To address this question, we analyzed the distribution of COPI by focusing on the beta -COP subunit. We observed a dramatic change in beta -COP distribution after peptide treatment. Vesicular structures containing beta -COP accumulated near the nucleus and in proximity to the Golgi complex. Similar results have been reported for anoxic pancreatic acinar cells (34). In those studies, ATP-depletion did not alter the Golgi stack but greatly reduced the number of ER to Golgi transport vesicles that were replaced by cytoplasmic, fibrillar aggregates containing beta -COP. These aggregates represent cytoplasmic pools of coatomer that self-associate after disruption of ER to Golgi traffic. Although like the anoxic condition the organization of the Golgi complex and the endoplasmic reticulum did not change after Rab2 peptide treatment, we observed a different beta -COP phenotype. Our studies show structures that overlapped when labeled with antibody to beta -COP, antibody to p58, and antibody to Rab2, indicating that the Rab2 peptide did not cause beta -COP membrane dissociation to the cytosol. On the contrary, we believe that VTCs are perpetually coated with COPI which interferes with subsequent trafficking through the Golgi complex. This result is similar to the effect produced by GTPgamma S when added to the intra-Golgi transport assay (35). In that case, coated vesicles and coated membranes form which cannot uncoat and inhibit subsequent fusion events necessary for intercisternal transport. Since VTCs in peptide-treated cells are "stalled," components are not retrieved from these structures that are necessary for cargo transport from the ER. Our previous observation that the Rab2 (13-mer) caused ts045 VSV-G to accumulate in punctate structures which were smaller and less abundant than VTCS that accumulate at 15 °C, supports this interpretation (2). We predict that prolonged incubation with the Rab2 peptide would ultimately result in complete inhibition of transport from the ER as well as recycling from pre-Golgi and Golgi compartments.

The results of our microsomal binding assay show that the Rab2 (13-mer) increased the rate and extent of COPI membrane association and that this enhanced recruitment is specific to the Rab2 peptide. We did not observe a similar level of beta -COP binding after incubation with a scrambled peptide or with amino-terminal peptides made to other Rab proteins. Interestingly, the Rab1B peptide and Rab2 peptide share 8 amino acids, yet the Rab1B peptide did not interrupt protein traffic (2) nor affect COPI recruitment. The ability of the Rab2 protein to promote beta -COP membrane association and the lack of recruitment by the Rab2Delta 14 protein supports our contention that the peptide functions as a bona fide Rab2 domain.

Combined biochemical and morphological data suggests that the peptide acts at a post-ER budding stage but before VSV-G exit from pre-Golgi structures. These structures segregate anterograde from retrograde-transported proteins, an event that requires the participation of ARF and coatomer (10). Our results indicate that ARF is necessary for Rab2 peptide and Rab2 protein-stimulated COPI binding. We suggest that ARF functions catalytically to facilitate Rab2 peptide and Rab2 protein enhancement of COPI binding. This requirement for ARF is consistent with the numerous publications showing ARF involvement in COPI recruitment (10, 21, 22). In particular, addition of an activated form of ARF (ARF1 Q71L) causes VSV-G to accumulate in pre-Golgi structures that contain beta -COP and p53/p58 (10). Furthermore, ARF1 can mediate the in vitro recruitment of the COPI coat to subcellular fractions enriched in cis Golgi/intermediate compartment membranes (26).

The Rab2 (13-mer) binds to membrane. However, the peptide did not interfere with Rab2 protein membrane association. Although it appears that the peptide is not a competive inhibitor for Rab2 protein membrane-binding sites, the Rab2 (13-mer) might influence Rab2 function by interaction with a downstream Rab2 effector. This effector could require interaction with the Rab2 amino terminus to regulate coat recruitment. The Rab2 peptide would therefore block the functional interaction of Rab2 with the downstream effector. This inhibition would lead to uncontrolled coatomer binding ultimately inhibiting vesicular traffic in the early secretory pathway. We have observed enhanced beta -COP recruitment when membranes are incubated with Rab2 protein and GTP (data not shown). However, a significant increase in beta -COP binding was obtained when GTPgamma S was included in the assay. The irreversible binding of the Rab2 protein to membrane mimics the irreversible nature of the Rab2 (13-mer). We propose that in steady state, Rab2 plays a role in coatomer recruitment to pre-Golgi intermediates (VTCs). This recruitment process requires PKC or a PKC-like protein.

Protein kinase C activity has been found in regulated (36) and constitutive exocytosis (31) and is required for receptor traffic through the endocytic path (37). All members of this family of isoenzymes have an amino-terminal regulatory domain that contains binding sites for phospholipid/diacylglycerol and calcium, and a carboxyl-terminal catalytic domain that binds ATP and has kinase activity (38). A variety of compounds are available which specifically bind to these domains and either activate or inhibit. These compounds allow one to determine if PKC exerts an effect independent of kinase activity. We evaluated the effect of calphostin C in the binding assay because PKC regulates ARF and COPI (30). Additionally, PKC inactivation by calphostin C arrests transport in the early secretory pathway before the site of Rab2 peptide inhibition (2, 39). Calphostin C binds to the PKC regulatory domain and blocks binding of diacylglycerol. In this study, calphostin C inhibited Rab2 (13-mer) and Rab2 protein stimulation of beta -COP membrane binding which indicates that PKC or a PKC-like protein functions upstream of the Rab2 protein. The kinase activity of this enzyme is not required based on the result that chelerythrine chloride which binds to the catalytic domain had no influence on beta -COP recruitment.

The role of PKC in mediating intracellular trafficking independent of phosphorylation has been reported for ER to Golgi transport (39) and in the production of post-Golgi vesicles (40). In both cases, a phorbol-ester binding protein was proposed to participate in the respective transport event. However, unlike the soluble phorbol ester-sensitive protein required for ER to Golgi transport, we believe that the PKC-like molecule required in Rab2 activity is membrane associated. Membranes preincubated with calphostin C, then pelleted and resuspended in cytosol and GTPgamma S do not bind beta -COP (data not shown). PKC isozymes are differentially expressed in tissue and cell-type and each translocate to a specific intracellular site upon activation by phorbol esters (41, 42). It is possible that the PKC-like molecule required for Rab2 activated beta -COP recruitment differs from the phorbol ester-binding protein that regulates exit from the ER.

The Proposed Role of Rab2 in the Secretory Pathway-- The phylogenetic tree of the Ras superfamily shows that Rab2 is most closely related to Rab4 which is interpreted to mean that these proteins are similar in function (43). Therefore, it is conceivable that the role of Rab2 in exocytosis is analogous to the role of Rab4 in endocytosis. In the endocytic pathway, Rab4 regulates the early recycling step from the "sorting endosome" to the plasma membrane (44-46). Since COPI-coated vesicles are involved in retrograde transport (13), the Rab2 protein may function in protein sorting and recycling events from pre-Golgi intermediates or "sorting exosomes" (7, 10). In this case, Rab2 would regulate vesicular traffic through a subcompartment within pre-Golgi elements. Such a subcompartment might function to sort and recycle escaped ER proteins that possess retrieval sequences. The recruitment of COPI to this subcompartment may result in vesicles that contain recycling proteins. The Rab4 protein plays a similar role in endocytosis by controlling a rate-limiting step in receptor transport from early endosomes to recycling endosomes (44).

    ACKNOWLEDGEMENT

We thank Dr. Nick Davis for criticial reading of the manuscript.

    FOOTNOTES

* This work was supported in part by American Cancer Society Research Grant ACS IN-162 (to E. J. T.).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.

§ To whom correspondence should be addressed. E-mail: etisdale{at}med.wayne.edu; Tel.: 313-577-1007; Fax: 313-577-6739.

1 The abbreviations used are: ER, endoplasmic reticulum; ARF, ADP-ribosylation factor; endo H, endoglycosidase H; PBS, phosphate-buffered saline; PKC, protein kinase C; VTC, vesicular tubular clusters; GTPgamma S, guanosine 5'-3-O-(thio)triphosphate; HRP, horseradish peroxidase; PAGE, polyacrylamide gel electrophoresis.

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Abstract
Introduction
Procedures
Results
Discussion
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