Correspondence to Julie G. Donaldson: jdonalds{at}helix.nih.gov
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Introduction |
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Arfs are expressed in all eukaryotes and function in various membrane trafficking events and in the maintenance of organelle structure (Moss and Vaughan, 1995; Chavrier and Goud, 1999). There are six mammalian Arfs, and Arf-1 and Arf-6 are the least similar in amino acid sequence and the best-characterized members of the Arf family. Arf-1 is primarily localized to the Golgi complex where it regulates the binding of cytosolic coat proteins, including coat protein I (COPI), adaptor protein 1, and Golgi-localized, -earcontaining, Arf-binding proteins (GGA) to Golgi membranes (Bonifacino and Lippincott-Schwartz, 2003; Nie et al., 2003) and thus serves to regulate membrane traffic in the ER-Golgi system (Lippincott-Schwartz et al., 1998). Arf-6, by contrast, localizes to the plasma membrane and a membrane recycling system at the cell periphery (Donaldson, 2003).
An important characteristic of Arf-1 is that the inactive protein (Arf-1-GDP) is largely cytosolic, whereas the activated protein (Arf-1-GTP) is membrane bound. Arf proteins are all myristoylated and it has been postulated that Arf-1-GDP initially docks on the membrane through this myristoyl moiety before encountering the guanine nucleotide exchange factor (GEF) that catalyzes exchange of GTP for GDP (Antonny et al., 1997). Arf-1-GTP associates more tightly with the membrane and can then recruit coat proteins to the membrane until it encounters a GTPase-activating protein (GAP) that stimulates GTP hydrolysis and dissociation of Arf-1-GDP from the membrane.
In biochemical assays, all Arf proteins share common effector functions including: activation of phospholipase D (Liang et al., 1997) and phosphatidylinositol 4-phosphate 5-kinase (Honda et al., 1999), recruitment of COPI to membranes (Liang and Kornfeld, 1997), and binding to GGA (Takatsu et al., 2002). Yet in cells, Arfs have distinct functions and localizations. Arf-1 localizes to the Golgi complex, regulates the assembly of coat proteins onto membranes and mediates traffic in the ER-Golgi system (Bonifacino and Glick, 2004). Arf-6 localizes to the endosomal/plasma membrane system and not the Golgi and thus has no effect on regulating the assembly of COPI onto the Golgi complex in vivo (Peters et al., 1995). Thus, it is through organelle-specific targeting that Arf proteins attain their unique cellular functions.
In this study, we were interested in identifying amino acid residues in the Arf-1 sequence that determine its specificity for Golgi targeting and distinguish it from other Arf proteins, especially Arf-6. Because Arf proteins are highly conserved in structure (Goldberg, 1998; Pasqualato et al., 2001), we followed an approach that has been used by us and others, generating chimeric Arfs by exchanging amino- and carboxy-terminal portions of Arf-1 and Arf-6 and expressing them in cells (Liang et al., 1997; Jones et al., 1999; Al-Awar et al., 2000). As a result of this study, we identified a short sequence in Arf-1 containing a Golgi targeting signal, and in the sequence we identified a motif (MXXE) that is critical in vitro and in vivo for Arf-1 binding to membrin, an ER-Golgi SNARE protein. Because the MXXE motif enables Arf-1 to localize to the early Golgi, we suggest that membrin is an Arf-1 receptor at the early Golgi.
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Results |
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Arf-6-1-6 and Arf-1-6-1 are activated by a BFA-sensitive GEF and inactivated by a GAP on the Golgi membrane
An important characteristic of Arf-1 is that the inactive, GDP-bound protein is in the cytosol whereas the active, GTP-bound protein is membrane bound, and cycling of Arf-1 between its activated and inactivated states is critical for Arf-1 function. When cells are treated with brefeldin A (BFA), a fungal toxin that inhibits Arf-GEFs that are associated with the Golgi complex (Jackson and Casanova, 2000), Arf-1 dissociates from Golgi membranes because activation of Arf-1 by GEF is inhibited, whereas GAP continues to inactivate Arf-1. To examine whether Arf-6-1-6 and Arf-1-6-1 can serve as substrates for GEFs and GAPs on the Golgi membrane like Arf-1, the dissociation of these Arf chimeras from the Golgi after addition of BFA were compared with that of Arf-1. In untreated COS-7 cells, clear Golgi localizations of Arf-6-1-6-GFP and Arf-1-6-1-GFP were observed (Fig. 2, Unt). After addition of BFA, both Arf-GFPs dissociated from the Golgi as rapidly as Arf-1-GFP (Fig. 2, BFA 2 min). These results show that both Arf-6-1-6 and Arf-1-6-1 can be inactivated through GTP hydrolysis by the GAP on the Golgi membrane. Furthermore, it suggests that activation of Arf-6-1-6 and Arf-1-6-1 is catalyzed by a BFA-sensitive Golgi GEF because neither Arf chimeras bound to the Golgi in the presence of BFA. Similar observations were made in HeLa cells (unpublished data).
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To test the possibility that those SNAREs act as Golgi membrane receptors for Arf-1 in mammalian cells, we coexpressed rbet1, sec22b, membrin, and syntaxin5, which are the mammalian homologues of Bet1p, Sec22p, Bos1p, and Sed5p, respectively, with Arf-1-GFP in HeLa cells. As reported (Hay et al., 1996, 1998), rbet1, membrin, and syntaxin5 mainly localized to the Golgi whereas sec22b localized to the ER. We noticed that, although Arf-1 generally colocalized with all of the Golgi-localized SNAREs (not depicted), Arf-1 localization was tightly coincident with membrin (Fig. 5 E), raising the possibility that Arf-1-GFP was directly binding to the overexpressed membrin and that membrin may be serving as an Arf-1 receptor in vivo.
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Having demonstrated that Arf-1 can specifically bind to solubilized membrin, we examined more carefully the extent of colocalization of Arf-1 and membrin in intact cells. In HeLa cells, we observed a high degree of colocalization between Arf-1 and membrin (Fig. 5 E). However, colocalization of Arf-1-6-1 with membrin was partial and some membrin-positive structures were clearly devoid of Arf-1-6-1 (Fig. 5 E, inset, arrowheads). We observed similar immunolocalization results in NRK cells where we quantified the amount of colocalization (see Materials and methods), and found that 80% of Golgi-associated Arf-1 colocalized with membrin whereas only 41% of Golgi-associated Arf-1-6-1 colocalized with membrin (Fig. 5 F). Importantly, if we mutated Arf-1-6-1 such that it now contained the MXXE motif, 75% colocalization between Arf-1-6-1MXXE and membrin was now observed (Fig. 5 F). We also observed near complete colocalization of membrin with GFP-Arf-1(101116) (unpublished data). These results suggest that Arf-1 can bind to membrin in vitro and in vivo but requires the MXXE motif. Arf-1-6-1, on the other hand, does not interact with membrin and thus must localize to the Golgi by an alternative mechanism.
The finding that Arf-1 could bind to membrin, both in cells and in in vitro binding assays, suggested that Golgi-associated membrin could act as the initial receptor for Arf-1-GDP before GEF-catalyzed nucleotide exchange. If this is true, it is possible that overexpression of membrin would partially protect Arf-1 from release from Golgi membranes during BFA treatment. When Arf-1 or Arf-1-6-1 was expressed alone in COS-7 cells, a significant amount of Arf dissociated from the Golgi within 2 min after BFA addition (Fig. 2, BFA 2 min). However, if membrin was coexpressed with Arf-1, Arf-1 labeling of the Golgi was still apparent after 2 min of BFA addition (Fig. 6 A). Even after 4 min, Golgi localization of Arf-1 was still prominent in membrin-transfected cells (Fig. 6 A, cell marked with arrowhead), whereas the bulk of the Arf-1 was dissociated in cells not coexpressing membrin (Fig. 6 A, cell marked with arrow). This association of Arf-1 with membrin was lost as Golgi membranes redistributed into the ER (see below). On the other hand, in Arf-1-6-1transfected cells, overexpressed membrin did not protect the dissociation of Arf-1-6-1 from the Golgi by BFA (Fig. 6 A), suggesting that the 16 aa of Arf-1 including the MXXE motif were required for this effect. Overexpression of membrin did not affect COPI dissociation after BFA addition (Fig. 6 B), indicating that "protection" of Arf-1 dissociation did not lead to GTP loading onto Arf-1. Because rbet1 and syntaxin5 also showed Golgi localization in mammalian cells, we examined whether overexpression of rbet1 or syntaxin5 would protect Arf-1 from dissociation by BFA. As shown in Fig. 6 C, regardless of the level of expression, neither rbet1 nor syntaxin5 affected the distribution of Arf-1 after BFA addition, indicating that overexpression of these SNAREs did not retain Arf-1 at the Golgi in COS-7 cells. We made similar observations in HeLa cells and quantified the amount of Arf-1 and Arf-1-6-1 associated with the Golgi before and after BFA in cells coexpressing these ER-Golgi SNAREs (Fig. 6, D and E). In untreated cells, 17% of total cellular Arf-1 was associated with the Golgi and this dropped to 6% after 2 min BFA (Fig. 6 D, control). In cells expressing membrin however, Arf-1 associated with the Golgi drops only to 12% after BFA (Fig. 6 D, +membrin). On the other hand, neither rbet1 nor syntaxin5 expression affected the distribution of Arf-1 after BFA addition (Fig. 6 D, +rbet1 and +syntaxin5). In Arf-1-6-1transfected cells, dissociation from the Golgi by BFA was similar in all cases and not affected by expression of any SNARE (Fig. 6 E). Together, these results indicate that membrin can specifically recruit Arf-1-GDP to Golgi membranes and transiently "protect" Arf-1-GDP from BFA-induced dissociation. Furthermore, that it is Arf-1-GDP that is binding to membrin is supported by the observation that Arf-1 Q71L did not colocalize with membrin in cells (unpublished data).
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In addition to GEFs, distinct GAPs may regulate Arf-1 at the Golgi in mammalian cells (Cukierman et al., 1995; Miura et al., 2002). It is likely that distinct GEFs and GAPs regulate Arf-1 at cis- and trans-elements of the Golgi complex. Having demonstrated that Arf-1-6-1 localizes mainly to the trans-Golgi, and not to the cis-Golgi, we wondered if Arf-1-6-1 is regulated differently from Arf-1. FRAP is a powerful technique to examine the kinetics of dissociation and association of Arf-1 at the Golgi in live cells (Vasudevan et al., 1998; Presley et al., 2002). Because the kinetics reflect GAP and GEF activities on Arf-1, we examined the FRAP of the Golgi region in Arf-1-GFP- and Arf-1-6-1-GFPtransfected cells. Representative FRAP kinetic data are shown in Fig. 9 A. The recovery of Arf-1-GFP fluorescence showed kinetics (t1/2 = 20 s) similar to previous studies (Presley et al., 2002). By contrast, the recovery kinetics of Arf-1-6-1-GFP (t1/2 = 10 s) was much more rapid, indicating that Arf-1-6-1 spends less time on the Golgi per cycle than Arf-1. Because Arf-1-6-1 primarily localizes to the late Golgi (Fig. 8), the difference in the FRAP data for Arf-1 and Arf-1-6-1 suggests that Arf-1 cycling at the trans-Golgi might be faster than at the cis-Golgi. We hypothesized that failure to bind to membrin at the early Golgi leads to Arf-1-6-1 being activated and inactivated at the late Golgi with more rapid kinetics. To test this, we measured the FRAP kinetics of Arf-1-6-1MXXE-GFP and observed that Arf-1-6-1MXXE-GFP now exhibited FRAP kinetics (t1/2 = 20 s) identical to that of wild-type Arf-1 (Fig. 9 A).
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Discussion |
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The first suggestion that ER-Golgi SNAREs could recruit Arf-1 came from in vitro binding studies in yeast (Rein et al., 2002) showing that nonmyristoylated, 17Arf1p-GDP could bind directly to GST fusion proteins of Bet1p, Sec22p, and Bos1p. In that study, Arf1p binding to Bet1p was stronger than to Bos1p and, curiously, required the presence of an Arf-GAP protein, Glo3p, to prime the SNAREs (Rein et al., 2002). Our study shows that membrin, but not rbet1, sec22b or syntaxin5, can bind specifically to full-length, myristoylated Arf-1 through the MXXE motif in mammalian cells. Because our cells express mammalian ArfGAP1, it is possible that this endogenous GAP could function in vivo to prime membrin for Arf-1 binding. Interestingly, the proximal region of helix
3 makes contact with ArfGAP1 in a co-crystal of
17Arf-1-GDP and the GAP domain of ArfGAP1 (Goldberg, 1999), raising the possibility that the recruitment of Arf-1 to the early Golgi by membrin might also involve ArfGAP1. Because yeast Arf1p also contains MXXE, and can be recruited to Golgi when expressed in mammalian cells (unpublished data), this motif may be used for Golgi targeting in yeast cells. Indeed, evidence that the
3 region in yeast promotes Golgi recruitment of Arf-1 comes from a genetic study that identified amino acid residues in the distal portion of helix
3 as an intragenic suppressor of a dominant lethal mutation (Click et al., 2002).
The other class of Golgi membrane proteins that have been suggested to serve as Arf-1 receptors are the abundant p23 and p24 family proteins. The p23 protein was shown by chemical cross-linking to bind directly to Arf-1-GDP, but not to Arf-1-GTP, in vitro and the interaction site was mapped to the carboxyl-terminal 22 aa (Gommel et al., 2001). Although this interaction was also observed in an in vivo study examining fluorescence resonance energy transfer between p23-CFP and Arf-1-YFP (Majoul et al., 2001), it may not represent the interaction that targets Arf-1-GDP specifically to the Golgi. We did not detect a Golgi targeting motif in the last 22 aa of Arf-1 because Arf-6-6-1, which lacked the 16amino acid sequence and the amino-terminal half of Arf-1 but contained Arf-1 sequence from 117181, did not localize to the Golgi (Fig. 1 D). Our data suggest that membrin serves as a specific receptor for Arf-1-GDP. However, it does not preclude an interaction of Arf-1-GDP with p23 proteins either simultaneously or subsequently during the interaction cycle of Arf-1 with Golgi membranes.
Arf proteins are highly conserved both in sequence and in structure with nearly identical switch I and II regions (Goldberg, 1998; Pasqualato et al., 2001). Helix 3 is positioned on the "backside" of the molecule, on the opposite side of the GTP binding pocket. It alone appears to contain sufficient information for Golgi targeting (Fig. 4) and presumably membrin binding. In the context of the Arf-1 protein, the MXXE motif in helix
3 appears to be required for Golgi targeting. We do not know whether the M or E make direct contact with membrin, but they are necessary for Arf-1 binding to membrin.
We propose that in the ER-Golgi system, membrin recruits Arf-1-GDP to the membrane subsequent to the release of the COPII coat (Fig. 9 B, I). Arf-1-GDP is then activated by GBF1, the early Golgi GEF, and Arf-1-GTP can then recruit coatomer or other effectors and Arf-GAP, leading to GTP hydrolysis and release of Arf-1-GDP back into the cytosol. The Arf-1 construct that cannot bind to membrin (Arf-1-6-1) can still associate with the Golgi complex, possibly by direct interaction with an Arf-GEF such as BIG1 and 2, which are known to reside at the trans-Golgi (Fig. 9 B, II; Shinotsuka et al., 2002a,b; Zhao et al., 2002). Arf-1-6-1 colocalizes less with GBF1 (Fig. 8, A and B) and, during recovery from BFA, Arf-1-6-1 cannot associate with the peripheral, COPI-labeled, reforming Golgi structures (Fig. 7 A). Intriguingly, we observed a distinct difference between the FRAP kinetics of Arf-1 and Arf-1-6-1 (Fig. 9 A). Namely, that Arf-1-6-1-GFP had a much shorter recovery time after photobleaching (t1/2 = 10 s) than did Arf-1-GFP (t1/2 = 20 s). We speculate that the shorter residency time for Arf-1-6-1 could be due to interaction with trans-Golgi GEFs (BIG1 and 2) and GAPs. In contrast, the residency time of Arf-1 on the Golgi is longer and includes interaction of Arf-1 with membrin, GBF1 and ArfGAP1 at early Golgi. These differences in kinetic cycles may reflect the different GEFs and GAPs residing at the early and late Golgi (Fig. 9 B, I, II).
Functional relationship between Arf-1 and SNAREs
SNAREs have an essential role in regulating membrane fusion events throughout the secretory pathway (Hay, 2001; Bonifacino and Glick, 2004). SNAREs form cytoplasmic coiled-coil bundles that bridge two membranes about to undergo membrane fusion. Furthermore, as SNAREs are compartment specific and can engage in various SNARE pair conformations, they have the potential to serve as exquisite membrane receptors for cytosolic components such as COPI and COPII components whose regulated assembly controls vesicle formation.
Current models for transport in the early secretory pathway depict secretory cargo and the SNAREs syntaxin5, rbet1, and membrin being recruited into COPII vesicle budding from the ER (Fig. 9 B, I; Springer and Schekman, 1998). Our observations that Arf-1 cannot bind to membrin when it is in the ER or at ER exit sites, i.e., 30 min BFA (Fig. 7) suggest that the altered conformation of membrin in the ER or association with the COPII coat may prevent Arf-1 binding. The tethering protein p115 associates with these newly budded vesicles by binding directly to the SNAREs in a Rab1-dependent fashion (Allan et al., 2000). At the Golgi, p115 and these SNAREs are believed to facilitate fusion of pre-Golgi structures to Golgi membranes or to other incoming pre-Golgi structures. GBF1 associates with p115 (Garcia-Mata and Sztul, 2003) and has been shown to be involved in COPI recruitment onto membranes (Claude et al., 1999; Kawamoto et al., 2002). Furthermore, GBF1 is essential for COPI recruitment to the transport intermediates bound for the Golgi (Garcia-Mata et al., 2003). These observations support the idea that p115 and membrin might coordinately recruit GBF1 and Arf-1-GDP onto the post-ER, transport structure, leading to Arf-1 activation and the recruitment of COPI (Fig. 9 B, I).
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Materials and methods |
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Plasmids and transient transfections
The chimeras of Arf-1 and Arf-6 were created by a two-step PCR procedure as described previously (Al-Awar et al., 2000). All other mutants of Arf-1 and Arf-6 were created using QuickChange site-directed mutagenesis kit (Stratagene). The cDNAs of untagged or carboxyl-terminally HA-tagged wild-type and mutant Arf were subcloned into the modified pCDL-SR expression vector (Takebe et al., 1988) or pEGFP-N1 vector (CLONTECH Laboratories, Inc.). Amino acids 101116 of Arf-1 were shuttled into pEGFP-C3 vector (CLONTECH Laboratories, Inc.). The plasmids for amino-terminally myc-tagged membrin, rbet1, sec22b, and HA-tagged syntaxin5 were created as described previously (Hay et al., 1996, 1997). The plasmids for GalT-GFP and HA-tagged GBF1 were provided by J. Lippincott-Schwartz (NIH; Cole et al., 1996) and C.L. Jackson, respectively.
Cells were grown on glass coverslips and transfected using FuGENE 6 (Roche) according to the manufacturer's instructions. For FRAP experiments, HeLa cells were plated in Lab-Tek chambered coverglass (Nalge Nunc International).
Confocal microscopy
20 h after transfection, cells were treated as indicated, fixed, and subjected to immunofluorescence staining in the presence of 0.2% saponin as described previously (Radhakrishna and Donaldson, 1997). All fluorescence images were obtained with a confocal microscope (model LSM 510; Carl Zeiss MicroImaging, Inc.). Most images of fixed cells were captured using 63x 1.4 NA objective with a pinhole corresponding to a focal depth of 0.7 µm. To quantify Golgi-associated Arf-1-GFP, a 40x 0.7 NA objective was used with a pinhole corresponding to a focal depth of 12.4 µm. For FRAP experiments, cells were incubated in CO2-independent media (Invitrogen), and imaged at 20°C on a confocal microscope (model LSM 510; Carl Zeiss MicroImaging, Inc.) using a 40x 0.7 NA objective with a pinhole corresponding to a focal depth of 2.5 µm. Image processing for figures was accomplished in Adobe Photoshop 5.5.
Analysis of colocalization
To quantify the level of colocalization for Golgi-associated Arfs with membrin, GBF1, and BIG1, 20 cells were randomly selected on the same coverslip. Levels for the laser power and detector amplification were optimized for each channel before starting the quantification. Images of the Golgi region were acquired at the same magnification and processed by Metamorph 4.6 (Universal Imaging Corp.).
In vitro binding experiments
To examine the interaction between His6-Arf-1 and membrin, HeLa cells overexpressing myc-membrin were lysed in binding buffer (25 mM Hepes, pH 7.5, 100 mM NaCl, 0.5 mM EDTA, 1 mM MgCl2, 1 mM DTT, 1 mM AEBSF, 3 µg/ml leupeptin, 3 µg/ml aprotinin, 3 µg/ml pepstatin A) containing 0.5% Triton X-100. Supernatants of the lysate were incubated with His6-tagged 17Arf-1 prebound to Ni-NTA beads (QIAGEN) in the presence of 1 mM GDP for 3 h at 4°C, and cross-linking reagent DSP was added at a final concentration of 1 mM. After incubation for 20 min at RT, DSP activity was quenched by addition of 50 mM glycine. The beads were washed and the proteins bound to beads were subjected to SDS-PAGE and immunoblot analysis with anti-myc antibody.
Online supplemental material
Fig. S1 shows that Arf-1-6-1 and Arf-1M110I, E113D when loaded with GTPS could bind to GST-VHS-GAT as well as wild-type Arf-1. Also, measurement of CD spectra of these Arf-1 mutants demonstrated that the general conformations of Arf-1-6-1 and Arf-1M110I, E113D are essentially identical to that of Arf-1. Fig. S2 shows that overexpressed GBF1 can activate Arf-1-6-1 in cells. Online supplemental material is available at http://www.jcb.org/cgi/content/full/jcb.200409138/DC1.
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Acknowledgments |
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A. Honda was supported by the JSPS Research Fellowships for Japanese Biomedical and Behavioral Researchers at NIH.
Submitted: 22 September 2004
Accepted: 16 February 2005
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