Mapping of Functional Domains of gamma -SNAP*

Katsuko Tani, Mika Shibata, Kazuho Kawase, Hoshiko Kawashima, Kiyotaka Hatsuzawa, Masami Nagahama, and Mitsuo TagayaDagger

From the School of Life Science, Tokyo University of Pharmacy and Life Science, Hachioji, Tokyo 192-0392, Japan

Received for publication, December 26, 2002

    ABSTRACT
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

gamma -Soluble N-ethylmaleimide-sensitive factor (NSF) attachment protein (gamma -SNAP) is capable of stabilizing a 20 S complex consisting of NSF, alpha -SNAP, and SNAP receptors (SNAREs), but its function in vesicular transport is not fully understood. Our two-hybrid analysis revealed that gamma -SNAP, unlike alpha -SNAP, interacts directly with NSF, as well as Gaf-1/Rip11, but not with SNAREs. Gaf-1/Rip11 is a gamma -SNAP-associated factor that belongs to the Rab11-interacting protein family. To gain insight into the molecular basis for the interactions of gamma -SNAP with NSF and Gaf-1/Rip11, we determined the regions of the three proteins involved in protein-protein interactions. gamma -SNAP bound to NSF via its extreme C-terminal region, and the full-length NSF was needed to interact with gamma -SNAP. Both the N-terminal and C-terminal regions of gamma -SNAP were required for the binding to Gaf-1/Rip11. Gaf-1/Rip11 bound to gamma -SNAP via its C-terminal domain comprising a putative coiled-coil region. Although the C-terminal domain of Gaf-1/Rip11 also interacts with Rab11, the binding of gamma -SNAP and Rab11 to Gaf-1/Rip11 was not mutually exclusive. Rather, Gaf-1/Rip11 was capable of serving a link between gamma -SNAP and Rab11. A complex comprising gamma -SNAP and Gaf-1/Rip11 was disassembled in a process coupled to NSF-mediated ATP hydrolysis, suggesting that the interaction between gamma -SNAP and Gaf-1/Rip11 is of functional significance.

    INTRODUCTION
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

Many membrane fusion events occurring in membrane trafficking in eukaryotic cells require a common set of proteins such as N-ethylmaleimide-sensitive factor (NSF)1 and SNAPs and membrane compartment-specific proteins consisting of complementary sets of coiled-coil proteins called SNAREs (1-4). Although the precise molecular mechanism for membrane fusion is not fully understood, one current model predicts that membrane fusion is driven by a tight binding between vesicle-associated SNAREs (the VAMP/synaptobrevin family) and target membrane-associated SNAREs (the syntaxin and SNAP-25 families) (5). SNAREs per se encode compartmental specificity of membrane fusion (6). Following membrane fusion, the cis (same membrane) SNARE complex is disassembled by the chaperone ATPase NSF (2). SNAPs not only serve as a linkage between NSF and the cis SNARE complex (7, 8) but also couple the energy produced by NSF-mediated ATP hydrolysis to a conformational change in syntaxin of the cis SNARE complex (9), which leads to the disassembly of the NSF-SNAPs-SNAREs complex (7, 8).

The SNAP family consists of ubiquitously expressed alpha  and gamma  isoforms and a brain-specific beta  isoform (10). So far alpha -SNAP has been studied most extensively. alpha -SNAP stimulates the ATPase activity of NSF (11) by interacting via its N-terminal and extreme C-terminal regions (12) and is essential for a wide variety of membrane fusion events including intra-Golgi protein transport (13). Based on the results of the x-ray crystallographic analysis of Sec17p, the yeast ortholog of alpha -SNAP (13, 14), it has been proposed that alpha -SNAP (Sec17p) functions as lever arms that transmit forces generated by a conformational change in NSF to SNAREs (15). Given the high sequence similarity between alpha -SNAP and beta -SNAP, it is postulated that the function of beta -SNAP is quite similar to that of alpha -SNAP. On the other hand, the physiological significance of gamma -SNAP is much less documented. Although gamma -SNAP enhances the secretion of neurotransmitters from several types of cells (16, 17), it exhibits a very low transport activity in an intra-Golgi protein transport assay (13) and is not required for transport from the endoplasmic reticulum to the Golgi (18). gamma -SNAP stabilizes the 20 S NSF-alpha -SNAP-SNAREs complex but cannot substitute for alpha -SNAP in complex formation (19).

Chen et al. (20) reported that Gaf-1 (gamma -SNAP-associated factor-1) encoded by the clone KIAA0857 (21) interacts with gamma -SNAP and is localized in the mitochondria. Independently, Prekeris et al. (22) demonstrated that the same protein but differently named Rip11 (Rab11-interacting protein), because of its ability to bind to Rab11, is localized in recycling endosomes and regulates apical membrane trafficking by interacting with Rab11 in polarized epithelial cells. Recent studies revealed that Gaf-1/Rip11 and several other proteins constitute a family of Rab11-interacting proteins (22-27).

In the present study we extensively characterized the interactions of gamma -SNAP with NSF and Gaf-1/Rip11. The results suggest that gamma -SNAP interacts with NSF via its extreme C-terminal region, whereas the N-terminal and C-terminal regions are required for the interaction with Gaf-1/Rip11. In addition, we showed a complex comprising gamma -SNAP and Gaf-1/Rip11 is disassembled in a process coupled to NSF-mediated ATP hydrolysis.

    EXPERIMENTAL PROCEDURES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
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DISCUSSION
REFERENCES

Antibodies-- A Gaf-1/Rip11 fragment (amino acids 524-653) and the full-length gamma -SNAP were expressed as His6-tagged proteins in Escherichia coli cells and purified using a nickel-nitrilotriacetic acid-agarose column (Qiagen). The isolated proteins were injected into rabbits to produce antisera. Monoclonal antibodies against Rab11 (clone 47; Transduction Laboratories), gamma -tubulin (GTU-88; Accurate Chemical and Scientific Co.), FLAG (M2; Sigma), and GST (Clontech) were obtained. A polyclonal antibody against GST was obtained from Santa Cruz Biotechnologies. A monoclonal antibody against c-Myc (clone 9E10) was purified from ascitic fluid and cross-linked to protein G beads using dimethyl pimelimidate. A monoclonal antibody against NSF (2E5) was prepared as described (28).

Plasmids-- pQE9, pQE30, and pQE31 were purchased from Qiagen and used for the expression of His6-tagged proteins. pGEX-4T-1 was obtained from Amersham Biosciences and used for the expression of GST fusion proteins. The clone KIAA0857 was obtained from the Kazusa DNA Research Institute, Kisarazu, Japan. pEBG (29) and pFLAG-CMV2 (Eastman Kodak Co.) were used for the expression of proteins in mammalian cells. The cDNA encoding gamma -SNAP was a generous gift from Dr. S. W. Whiteheart (University of Kentucky College of Medicine). The plasmids for Myc-tagged Rab11Q70L and Rab11S25N were kindly donated by Dr. Y. Takai (Osaka University).

Two-hybrid Analysis-- The full-length cDNA of gamma -SNAP was inserted into pGBT9, and the resultant plasmid was used as bait. A GAL4 DNA activation domain fusion library in pACT2 (MATCHMAKER human kidney cDNA library; Clontech) was used to isolate interacting clones. Yeast colonies that grew in medium lacking histidine were picked up, and their beta -galactosidase activity was assayed on filters. To examine protein-protein interactions, cDNAs for gamma -SNAP and alpha -SNAP were inserted into the bait plasmid pGBT9, and cDNAs for NSF and Gaf-1/Rip11 were inserted into the prey plasmid pGAD424. beta -Galactosidase activity was measured after transformation of yeast with the indicated combinations of the bait and prey plasmids.

Pull-down Experiments Using Recombinant Proteins-- Recombinant GST proteins were mixed with 10 µl of glutathione-Sepharose 4B and then the mixture was gently rotated at 4 °C for 30 min. After the beads were washed, they were incubated with His6-tagged proteins in incubation buffer comprising 20 mM HEPES/KOH, pH 7.0, 50 mM KCl, 2 mM mercaptoethanol, 0.5 mM ATP, 10% glycerol, and 1 mg/ml bovine serum albumin at 4 °C for 1 h with gentle rotation. The beads were washed three times with incubation buffer devoid of bovine serum albumin, and the bound proteins were eluted with 50 mM Tris-HCl, pH 8.0, with 5 mM glutathione. The eluted proteins were concentrated by trichloroacetic acid-deoxycholate precipitation and then subjected to SDS-PAGE on 10% gels. Gels were stained with Coomassie Brilliant Blue R-250.

Immunoprecipitation and Pull-down Experiments in a Mammalian Expression System-- Transfection of cells and preparation of cell lysates were performed as described (30). For co-transfection, plasmids (1 µg each) were used. At 20 h after transfection, cells plated on 35-mm dishes were washed and then lysed in 300 µl of lysis buffer comprising 25 mM HEPES/KOH, pH 7.2, 1% Triton X-100, 150 mM KCl, 0.5 µg/ml leupeptin, 2 µM pepstatin, 2 µg/ml aprotinin, 2 mM EDTA, 1 mM phenylmethylsulfonyl fluoride, and 1 mM dithiothreitol. The lysates were clarified by centrifugation. To the supernatants was added 3-5 µg of an antibody. After 30 min on ice, 10 µl of protein G-Sepharose 4B was added to the mixtures and then incubated at 4 °C for 2 h with gentle rotation. The beads were washed with lysis buffer several times and then the bound proteins were eluted by boiling in 10 µl of 2× SDS-PAGE sample buffer. For pull-down experiments, cell lysates were mixed with 10 µl of glutathione-Sepharose 4B and then incubated at 4 °C for 2 h with gentle rotation. The beads were washed, and the bound proteins were eluted as described above.

Immunoblotting-- Proteins were separated by SDS-PAGE and then transferred to nitrocellulose membranes. After incubation with appropriate primary antibodies and then with horseradish peroxidase-conjugated secondary antibodies, the membranes were developed on autoradiographic film by enhanced chemiluminescence (Amersham Biosciences).

Preparation of Rat Liver Membranes-- Livers were removed from starved rats, rinsed, perfused, and weighed. They were cut into small pieces and homogenized with a Potter-Elvehjem homogenizer (5 strokes) in 4 volumes of homogenization buffer comprising 25 mM HEPES/KOH, pH 7.2, 100 mM KCl, 0.5 µg/ml leupeptin, 2 µM pepstatin, 2 µg/ml aprotinin, 2 mM EDTA, 1 mM phenylmethylsulfonyl fluoride, and 1 mM dithiothreitol. The homogenate was centrifuged at 3,000 rpm (Tomy TA-4 rotor) for 10 min and then at 10,000 rpm for 10 min. The supernatant was centrifuged at 33,000 rpm (Beckman 50.2Ti rotor) for 1 h to recover membranes.

Velocity Sedimentation-- Velocity sedimentation was performed essentially as described (7) with a slight modification. Rat liver membranes (1.0 mg) were solubilized with 1% Triton X-100, and insoluble materials were removed by centrifugation. The membrane extracts (220 µl) were mixed with His6-tagged NSF (3 µg) and His6-tagged gamma -SNAP (0.7 µg), and the mixture was incubated on ice for 30 min. When indicated, 1 M MgCl2 was added to the mixture at a final concentration of 8 mM. The mixture was layered on the top of glycerol gradients consisting of 0.4 ml each of gradient buffer containing 35, 32.5, 30, 27.5, 25, 22.5, 20, 17.5, 15, and 12.5% glycerol (w/v). After centrifugation at 34,000 rpm (Beckman SW50 rotor) for 13 h, fractions (0.4 ml each) were recovered from the top. The proteins of the gradient fractions were precipitated with trichloroacetic acid and deoxycholate, washed with acetone, and then dissolved in SDS-PAGE sample buffer.

Disassembly of a Complex Containing GST-Gaf-1/Rip11 and gamma -SNAP-- Cells expressing GST-Gaf-1/Rip11 and FLAG-tagged gamma -SNAP, cultured on 35-mm dishes, were lysed in 300 µl of lysis buffer. The lysates were mixed with an equal volume of cell lysates separately prepared from non-transfected cells. When indicated, 1 M MgCl2 was added to the mixture at a final concentration of 8 mM. The mixture was incubated at 16 °C for 1 h and then GST-Gaf-1/Rip11 was pulled down with glutathione beads. The proteins pulled down were subjected to SDS-PAGE and analyzed by immunoblotting with antibodies against GST and FLAG.

For the preparation of NEM-treated cell lysates, non-transfected cells were lysed in lysis buffer devoid of dithiothreitol. The cell lysates were incubated with 1 mM NEM on ice for 15 min followed by 15 min treatment with 2 mM dithiothreitol to quench excess NEM.

    RESULTS
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
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DISCUSSION
REFERENCES

Screen of gamma -SNAP-interacting Proteins-- To identify gamma -SNAP-interacting proteins other than Gaf-1/Rip11 (20), we screened a human kidney expression library using the full-length gamma -SNAP as bait. Screening two times yielded 68 positive clones. Among the clones obtained, 20 clones encoded Gaf-1/Rip11, and 24 appeared to encode its alternative splice variant, because the encoded protein possesses the same C-terminal 131 amino acid residues as Gaf-1/Rip11 but has a different N-terminal sequence. Characterization of the putative splice variant will be described elsewhere. Fifteen clones were found to comprise the entire coding region of NSF. Proteins encoded by the other nine clones were different from one another. One was cytosolic thiolase, which was also identified as a potential gamma -SNAP-interacting protein in a two-hybrid screen by Chen et al. (20).

Interaction between gamma -SNAP and NSF-- Because the direct interaction between gamma -SNAP and NSF was not reported previously, we decided to analyze the interaction in detail. We first generated gamma -SNAP mutants encoding the N-terminal half (amino acids 1-152) and the C-terminal one (amino acids 153-312). A two-hybrid assay revealed that the C-terminal region is responsible for the interaction with NSF (Fig. 1A). We then generated a series of mutants with C-terminal deletions. When two amino acids were removed from the C terminus, the interaction between gamma -SNAP and NSF was abolished. To examine whether the two C-terminal residues, Leu-311 and Cys-312, directly contribute to the interaction with NSF, we replaced them individually and both by Ala via site-directed mutagenesis. The results showed that both the residues are important for the interaction with NSF (Fig. 1A).


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Fig. 1.   Mapping of the binding site for NSF on gamma -SNAP. A, two-hybrid analysis. Full-length or mutant gamma -SNAP cDNA fragments and full-length NSF cDNA were inserted into pGBT9 and pGAD424, respectively. The interaction of gamma -SNAP or its mutants with NSF in yeast was examined using a beta -galactosidase filter assay. B, pull-down experiments. Coomassie-stained gel of isolated His6-tagged NSF (lane 1), GST (lane 2), GST-gamma -SNAP (full-length; gamma -SNAP(F)) (lane 3), GST-gamma -SNAP (amino acids 1-152; gamma -SNAP(N)) (lane 4), and GST-gamma -SNAP (amino acids 153-312; gamma -SNAP(C)) (lane 5). To analyze protein-protein interactions, His6-tagged full-length NSF (10 µg) was mixed with glutathione-Sepharose 4B that had been incubated with 12 µg of GST (lane 6), GST-gamma -SNAP (full-length) (lane 7), GST-gamma -SNAP (amino acids 1-152) (lane 8), or GST-gamma -SNAP (amino acids 153-312) (lane 9). The bound proteins were eluted with glutathione, separated by SDS-PAGE, and stained. C, pull-down experiments. Coomassie-stained gel of isolated NSF (lane 1), GST (lane 2), GST-gamma -SNAP (wild-type) (lane 3), GST-gamma -SNAP mutant in which Leu-311 was replaced by Ala (L311A; lane 4), and GST-gamma -SNAP mutant in which Cys-312 was replaced by Ala (C312A; lane 5). To analyze protein-protein interactions, His6-tagged full-length NSF (10 µg) was mixed with glutathione-Sepharose 4B that had been incubated with 12 µg of GST (lane 6), GST-gamma -SNAP (wild-type) (lane 7), GST-gamma -SNAP (L311A) (lane 8), or GST-gamma -SNAP (C312A) (lane 9). The bound proteins were eluted with glutathione, separated by SDS-PAGE, and stained.

To confirm the results of the two-hybrid analysis, we performed an in vitro binding assay using isolated bacterial proteins. To facilitate purification, NSF was expressed as a His6-tagged protein, and gamma -SNAP was expressed as a GST fusion protein. Consistent with the results of the two-hybrid analysis, His6-tagged NSF was pulled down with GST-gamma -SNAP (full-length) (Fig. 1B, lane 7) and GST-gamma -SNAP (amino acids 153-312) (lane 9) but not with GST-gamma -SNAP (amino acids 1-152) (lane 8). In addition, His6-tagged NSF was not pulled down with GST-gamma -SNAP in which Leu-311 was replaced by Ala (L311A) (Fig. 1C, lane 8). Although His6-tagged NSF was pulled down with GST-gamma -SNAP in which Cys-312 was replaced by Ala (C312A) (lane 9), the amount was smaller than that pulled down with wild-type GST-gamma -SNAP. These results clearly showed that the extreme C-terminal region, especially Leu-311, is important for the interaction with NSF.

We next determined the binding site for gamma -SNAP on NSF. NSF can be divided into three domains, N-terminal and two ATP-binding domains referred to as D1 and D2 (28, 31, 32). Two-hybrid analysis and in vitro binding experiments revealed that the full-length NSF, but neither the N-terminal domain (amino acids 1-205) nor the D1D2 domain (amino acids 206-744), binds to gamma -SNAP (Fig. 2). These results are consistent with the fact that only full-length NSF clones were obtained in the two-hybrid screen.


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Fig. 2.   Full-length NSF is required for the interaction with gamma -SNAP. A, two-hybrid analysis. Full-length gamma -SNAP cDNA and full-length or truncated NSF cDNA fragments were inserted into pGBT9 and pGAD424, respectively. The interaction of gamma -SNAP with NSF or its fragments in yeast was examined using a beta -galactosidase filter assay. B, pull-down experiments. Coomassie-stained gel of isolated His6-tagged NSF (lane 1), the N-domain (amino acids 1-205; lane 2), the D1D2 domain (amino acids 206-744; lane 3), GST (lane 4), and GST-gamma -SNAP (lane 5). To analyze protein-protein interactions, 10 µg of His6-tagged full-length NSF (lanes 6 and 7), the N-domain (lane 8), or the D1D2-domain (lane 9) was mixed with glutathione-Sepharose 4B that had been incubated with 12 µg of GST (lane 6) or GST-gamma -SNAP (full-length) (lanes 7, 8, and 9). The bound proteins were eluted with glutathione, separated by SDS-PAGE, and stained.

gamma -SNAP Does Not Bind to SNAREs-- alpha -SNAP interacts primarily with syntaxin and weakly with SNAP-25 (9, 33). Our previous results (34) demonstrated that SNAREs can interact with alpha -SNAP in the yeast two-hybrid system even though they possess membrane anchors. The fact that clones encoding SNAREs were not obtained in the two-hybrid screen using gamma -SNAP as bait may suggest that gamma -SNAP does not interact directly with SNAREs. Indeed, a two-hybrid assay demonstrated that gamma -SNAP does not interact with various syntaxins, cellubrevin (a ubiquitously expressed protein of the VAMP-2 family) (35), or SNAP-23 (a ubiquitously expressed protein of the SNAP-25 family) (36) (Table I). These observations raised the possibility that gamma -SNAP is incorporated into the NSF-alpha -SNAP-SNAREs complex through binding to NSF. To test this possibility, we carried out velocity sedimentation analysis. Triton X-100 extracts of rat liver membranes were incubated with purified recombinant His6-NSF and His6-gamma -SNAP in the presence or absence of Mg2+-ATP, and the mixtures were then subjected to velocity centrifugation. As shown in Fig. 3A, significant amounts of endogenous and recombinant His6-gamma -SNAP co-sedimented with NSF in the absence of Mg2+ (fractions 7-9). In contrast, no co-sedimentation was observed in the presence of Mg2+ (Fig. 3B). These results were essentially the same as those reported previously (7). In the case of a gamma -SNAP mutant (L311A) that is defective in the ability to bind to NSF, no co-sedimentation with NSF was observed even in the absence of Mg2+ (Fig. 3C), suggesting that the interaction with NSF is essential for gamma -SNAP to be incorporated into the 20 S complex.


                              
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Table I
Interaction between SNAPs and SNAREs in the two-hybrid system
alpha -SNAP and gamma -SNAP were inserted into pGBT9 (bait plasmid), and SNAREs were inserted into pGAD424 (prey plasmid). After co-transformation of yeast with the indicated combinations of the bait and prey plasmids, beta -galactosidase activity was measured.


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Fig. 3.   gamma -SNAP is incorporated into a 20 S complex through binding to NSF. Triton X-100 extracts of rat liver membranes were incubated with His6-tagged NSF and His6-tagged gamma -SNAP in the absence (A) or presence (B) of MgCl2 and then subjected to velocity sedimentation analysis. Alternatively, the extracts were incubated with His6-tagged NSF and a His6-tagged gamma -SNAP mutant (L311A) in the absence of MgCl2 (C). After centrifugation, the proteins in each fraction were precipitated, separated by SDS-PAGE, and analyzed by immunoblotting with anti-NSF and anti-gamma -SNAP antibodies. NSF in fractions 2-4 may represent partially unfolded or degraded ones. NSF sedimented more slowly in the presence of Mg2+ (B) than its absence (A), reflecting the disassembly of the NSF-SNAPs-SNAREs complex in the presence of Mg2+. Two major bands recognized by the anti-gamma -SNAP antibody correspond to His6-tagged gamma -SNAP (slower migrating band on gels) and endogenous gamma -SNAP (faster migrating band on gels), respectively. Note that the gamma -SNAP mutant did not co-sediment with NSF in the absence of Mg2+, whereas the endogenous one did (C).

Interaction between gamma -SNAP and Gaf-1/Rip11-- To gain insight into the mechanism governing the interaction between gamma -SNAP and Gaf-1/Rip11, we determined the region of Gaf-1/Rip11 involved in the association with gamma -SNAP. The binding site for gamma -SNAP on Gaf-1/Rip11 must be within its C-terminal 131 amino acids, because the C-terminal region common to Gaf-1/Rip11 and its putative alternative splice variant interacts with gamma -SNAP in the two-hybrid system. We constructed a series of C-terminal fragments of Gaf-1/Rip11 and performed a yeast two-hybrid assay using the full-length gamma -SNAP as bait (Fig. 4A). The results confined the region responsible for the interaction with gamma -SNAP to amino acids 590-640 of Gaf-1/Rip11. This region comprises a putative coiled-coil region (amino acids 608-640), but the coiled-coil region alone was not sufficient to interact with gamma -SNAP. To confirm this observation, we constructed plasmids to express amino acids 590-640 and 608-640 of Gaf-1/Rip11 as GST fusion proteins and gamma -SNAP as a FLAG-tagged protein and performed pull-down experiments after co-transfection of the plasmids into 293T cells (Fig. 4B). Consistent with the results of the yeast two-hybrid analysis, FLAG-tagged gamma -SNAP was pulled down with the GST fusion protein comprising amino acids 590-640 of Gaf-1/Rip11 (lane 6) but not with that comprising amino acids 608-640 (lane 5).


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Fig. 4.   The C-terminal region common to Gaf-1/Rip11 and its alternative splice variant is involved in the interaction with gamma -SNAP. A, two-hybrid analysis. Full-length gamma -SNAP cDNA and full-length or truncated Gaf-1/Rip11 cDNA fragments were inserted into pGBT9 and pAD424, respectively. The interaction between gamma -SNAP and Gaf-1/Rip11 or truncated ones in yeast was examined using a beta -galactosidase filter assay. C2 represents the C2-domain. Hatched and filled boxes denote the C-terminal region common to Gaf-1/Rip11 and its alternative splice variant and the putative coiled-coil region, respectively. B, interaction between gamma -SNAP and truncated Gaf-1/Rip11 constructs in mammalian cells. 293T cells were transfected with a plasmid encoding GST (lanes 1 and 4) or a Gaf-1/Rip11 fragment corresponding to amino acids 608-640 (lanes 2 and 5) or 590-640 (lanes 3 and 6) fused to GST, in addition to a plasmid for FLAG-tagged gamma -SNAP. The GST fusion proteins in cell lysates were pulled down, and the precipitated proteins were analyzed by immunoblotting with antibodies against gamma -tubulin, FLAG, and GST (lanes 4-6). Five percent input was also analyzed (lanes 1-3).

A previous study revealed that Gaf-1/Rip11 is associated with gamma -tubulin (20). Interestingly, endogenous gamma -tubulin was efficiently pulled down with the construct comprising amino acids 608-640, which could not interact with gamma -SNAP, suggesting that this region is sufficient to interact with gamma -tubulin. The fact that the amount of gamma -tubulin bound to the construct containing amino acids 590-640 of Gaf-1/Rip11 was trivial compared with that bound to the construct containing amino acids 608-640 may imply that expressed FLAG-tagged gamma -SNAP competed with endogenous gamma -tubulin for the binding to the construct containing amino acids 590-640 of Gaf-1/Rip11.

To determine the region of gamma -SNAP involved in the interaction with Gaf-1/Rip11, we performed a two-hybrid assay using gamma -SNAP or its deletion mutants as bait. The results are summarized in Fig. 5A. Deletion of N-terminal 23 amino acids or C-terminal 89 amino acids eliminated the interaction with Gaf-1/Rip11. Similar results were obtained when pull-down experiments were conducted using a mammalian expression system (Fig. 5B).


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Fig. 5.   Mapping of the Gaf-1/Rip11-binding sites on gamma -SNAP. A, two-hybrid analysis. Full-length or truncated gamma -SNAP cDNA fragments and full-length Gaf-1/Rip11 were inserted into pGBT9 and pGAD424, respectively. The interaction of gamma -SNAP or truncated ones with Gaf-1/Rip11 in yeast was examined using a beta -galactosidase filter assay. Although two gamma -SNAP fragments (amino acids 1-245 and 1-268) exhibited weak positive signals in the absence of the prey vector, their signals were considerably stronger in the presence of the prey vector. B, interaction of gamma -SNAP or its mutants with Gaf-1/Rip11 in mammalian cells. 293T cells were co-transfected with plasmids for GST-Gaf-1/Rip11 and FLAG-tagged full-length gamma -SNAP (lanes 1 and 8) or fragments corresponding to amino acids 10-312 (lanes 2 and 9), 24-312 (lanes 3 and 10), 1-223 (lanes 4 and 11), 1-245 (lanes 5 and 12), 1-268 (lane 6 and 13), or 1-295 (lanes 7 and 14). GST-Gaf-1/Rip11 in cell lysates was pulled down, and the precipitated proteins were analyzed by immunoblotting with antibodies against GST and FLAG (lanes 8-14). Two percent input was also analyzed (lanes 1-7).

Gaf-1/Rip11 Is Able to Link gamma -SNAP to Rab11-- Members of the Rab11-interacting protein family share a highly conserved region of 20 amino acids at the C terminus (22-26). Prekeris et al. (23) showed that a peptide corresponding to amino acids 628-645 of Gaf-1/Rip11 competes with Gaf-1/Rip11 protein for the binding to Rab11. Because the Rab11-binding domain on Gaf-1/Rip11 markedly overlaps with the gamma -SNAP-binding domain, we wondered whether the gamma -SNAP-binding domain can interact with Rab11. Myc-tagged Rab11 proteins and the full-length Gaf-1/Rip11 or its fragments fused to GST were expressed in 293T cells, and immunoprecipitation was performed by using an anti-Myc antibody. As shown in Fig. 6A, the gamma -SNAP-binding domain (amino acids 590-640 of Gaf-1/Rip11) can interact with the constitutively active Rab11, Rab11Q70L (lane 9), although its interaction was markedly weaker than the interaction of the full-length Gaf-1/Rip11 (lane 10). Perhaps the C-terminal sequence (amino acids 641-645) of the Rab11-binding domain significantly contributes to the binding to Rab11. No interaction was observed with the inactive Rab11, Rab11S25N (lane 12). The coiled-coil region responsible for the interaction with gamma -tubulin (amino acids 608-640 of Gaf-1/Rip11) did not bind to Rab11Q70L (lane 8).


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Fig. 6.   Interaction between Gaf-1/Rip11 and Rab11. A, the C-terminal region of Gaf-1/Rip11 is involved in the interaction with Rab11. 293T cells were transfected with a plasmid encoding GST (lane 1), Gaf-1/Rip11 fragment corresponding to amino acids 608-640 (lanes 2 and 5), 590-640 (lanes 3 and 6), or full-length Gaf-1/Rip11 (lane 4) fused to GST, in addition to a plasmid encoding Rab11Q70L (lanes 1-4) or Rab11S25N (lanes 5 and 6) tagged with Myc. The expression levels of Myc-tagged Rab proteins were comparable (data not shown). Myc-tagged Rab proteins were immunoprecipitated, and the precipitated proteins were analyzed by immunoblotting with an anti-GST antibody (lanes 7-12). Five percent input was also analyzed (lanes 1-6). HC and LC denote immunoglobulin heavy chain and light chain, respectively. B, Gaf-1/Rip11 can link Rab11 to gamma -SNAP. 293T cells were co-transfected with plasmids for Gaf-1/Rip11 (lanes 1, 2, 5, and 6), Myc-tagged Rab11Q70L (lanes 1, 3, 5, and 7) or Rab11S25N (lanes 2, 4, 6, and 8), and FLAG-tagged gamma -SNAP (lanes 1-8). Myc-tagged Rab proteins were immunoprecipitated with an anti-Myc antibody cross-linked to protein G beads, and the precipitated proteins were analyzed by immunoblotting with antibodies against Gaf-1/Rip11, FLAG, and Myc (lanes 5-8). Five percent input was also analyzed (lanes 1-4).

Given that Rab11 and gamma -SNAP occupy the same region on Gaf-1/Rip11, we predicted that gamma -SNAP inhibits the binding of Rab11 to Gaf-1/Rip11 in a competitive manner. However, when Myc-tagged Rab11Q70L, Gaf-1/Rip11, and FLAG-tagged gamma -SNAP were co-expressed, Gaf-1/Rip11 was still co-precipitated with an anti-Myc antibody (Fig. 6B, lane 5). Surprisingly, a small but significant amount of FLAG-tagged gamma -SNAP was also co-precipitated with Myc-Rab11Q70L. On the other hand, no co-precipitation of FLAG-tagged gamma -SNAP was observed with Myc-Rab11S25N even in the presence of Gaf-1/Rip11 (lane 6). It should be noted that expression of Gaf-1/Rip11 is prerequisite for the co-precipitation of gamma -SNAP with Rab11Q70L (lane 7). These results suggest that Gaf-1/Rip11 is able to link between Rab11 and gamma -SNAP, although the linkage efficiency is not high.

A Complex Containing gamma -SNAP and Gaf-1/Rip11 Is Disassembled in a Mg2+-ATP-, NSF-dependent Manner-- The 20 S NSF-SNAPs-SNAREs complex is disassembled in a process coupled to NSF-mediated ATP hydrolysis (7). This most likely reflects disassembly of the cis SNARE complex after membrane fusion (1-4). We were interested in whether the binding between gamma -SNAP and Gaf-1/Rip11 is also affected by NSF and alpha -SNAP in a Mg2+-ATP-dependent manner. To address this question, Triton X-100 extracts prepared from cells expressing FLAG-tagged gamma -SNAP and GST-Gaf-1/Rip11 were mixed with lysates separately prepared from non-transfected cells, and the mixtures were incubated in the presence of EDTA-ATP or Mg2+-ATP. GST-Gaf-1/Rip11 in the mixtures was pulled down, and the precipitated proteins were analyzed by immunoblotting. As shown in Fig. 7, addition of Mg2+-ATP caused the dissociation of FLAG-tagged gamma -SNAP from GST-Gaf-1/Rip11 (lane 9), implying the disassembly of the gamma -SNAP-Gaf-1/Rip11 complex. Addition of cell lysates from non-transfected cells was necessary for efficient disassembly. It should be noted that FLAG-tagged gamma -SNAP and GST-Gaf-1/Rip11 were overexpressed. Perhaps the cell lysates may supply membrane and cytosolic proteins required for the disassembly reaction under conditions in which gamma -SNAP and Gaf-1/Rip11 were present at high levels. When cell lysates were pretreated with 1 mM NEM, no dissociation of FLAG-tagged gamma -SNAP from GST-Gaf-1/Rip11 occurred (lane 13), indicating the requirement of NEM-sensitive component(s) for this process. Addition of His6-tagged NSF and His6-tagged alpha -SNAP restored the dissociation reaction (lane 15). These results unequivocally showed the requirement of NSF for the disassembly of the gamma -SNAP-Gaf-1/Rip11 complex.


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Fig. 7.   NSF-mediated disassembly of the gamma -SNAP-Gaf-1/Rip11 complex. Lysates from cells expressing FLAG-tagged gamma -SNAP and GST-Gaf-1/Rip11 were mixed with non-transfected cell lysates (lanes 1-4 and 9-12) or NEM-treated lysates of non-transfected cells (lanes 5-8 and 13-16). The mixture was incubated in the presence of EDTA-ATP (lanes 2, 4, 6, 8, 10, 12, 14, and 16) or Mg2+-ATP (lanes 1, 3, 5, 7, 9, 11, 13, and 15) without (lanes 1, 2, 5, 6, 9, 10, 13, and 14) or with 0.5 µg of His6-tagged NSF and 0.5 µg of His6-tagged alpha -SNAP (lanes 3, 4, 7, 8, 11, 12, 15, and 16). GST-Gaf-1/Rip11 was pulled down, and the precipitated proteins were analyzed by immunoblotting with antibodies against GST and FLAG (lanes 9-16). Two percent input was also analyzed (lanes 1-8).


    DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES

In the present study we analyzed the interactions of gamma -SNAP with NSF and Gaf-1/Rip11 in detail using the yeast two-hybrid system and isolated recombinant proteins or a mammalian expression system. Our results demonstrated that the extreme C-terminal region of gamma -SNAP, especially Leu-311, is required for the interaction with NSF, and the N-terminal 23 amino acids and C-terminal 89 amino acids of gamma -SNAP contribute to the binding to Gaf-1/Rip11. For the interaction with gamma -SNAP, on the other hand, the entire coding region of NSF and the C-terminal region (amino acids 590-640) of Gaf-1/Rip11 are required.

Although alpha -SNAP mediates the attachment of NSF to SNAREs (7, 8), it appears that alpha -SNAP interacts with NSF only when it binds to SNAREs or plastic (12, 13, 37). Binding of alpha -SNAP to plastic may cause a conformational change in alpha -SNAP similar to that occurring upon binding to SNAREs. Consistent with the idea that SNAREs are required for the interaction of alpha -SNAP with NSF, no clones encoding NSF were obtained in our previous two-hybrid screen using alpha -SNAP as bait (34). Indeed, our yeast two-hybrid assay showed that alpha -SNAP hardly interacts with NSF (data not shown). In contrast, gamma -SNAP interacts with NSF in the absence of SNAREs. Despite this difference in the interactions between the two species of SNAPs and NSF, the penultimate leucine residues of the SNAPs (Leu-294 in alpha -SNAP and Leu-311 in gamma -SNAP) are important for the binding to NSF. In comparison with alpha -SNAP, gamma -SNAP appears to have a 22-amino acid insertion between the putative C-terminal alpha -helix, which corresponds to loop alpha 14 in Sec17p (15), and the penultimate leucine. This extra sequence may shift the position of Leu-311 such that it can interact with NSF in the absence of SNAREs. Interestingly, replacements of the penultimate leucine residues cause opposite effects in terms of the binding to NSF. An alpha -SNAP mutant in which Leu-294 is replaced by Ala is able to interact with NSF in a 20 S complex but unable to fully disassemble the complex in the presence of Mg2+-ATP (12). In contrast, the corresponding gamma -SNAP mutant is unable to bind to NSF.

Gaf-1/Rip11 is a member of the recently identified Rab11-interacting protein family (22-27). The highly conserved C-terminal region of Rab11-interacting protein family members is responsible for the binding to Rab11. In the present study we revealed that the same or markedly overlapping region is capable of interacting with gamma -SNAP. Despite the fact that Rab11 and gamma -SNAP bind to the overlapping site on Gaf-1/Rip11, overexpression of gamma -SNAP did not inhibit the binding of expressed Rab11 to Gaf-1/Rip11. Rather, a significant amount of gamma -SNAP was co-precipitated with Rab11 in the presence of Gaf-1/Rip11, suggesting that Gaf-1/Rip11 is able to serve as a link between gamma -SNAP and Rab11. How can Gaf-1/Rip11 connect gamma -SNAP to Rab11? Members of the Rab11-interacting protein family including Gaf-1/Rip11 are known to possess extensive homo- and hetero-interacting abilities (27). Using these abilities Gaf-1/Rip11 may constitute a scaffold or a hydrophobic patch (38) that can accommodate Rab11 and gamma -SNAP. Obviously, members of the Rab11-interacting protein family bind many proteins. Rab11-FIP2, a member of the family, interacts not only with Rab11 but also with proteins involved in recycling and endocytosis such as myosin Vb, Reps1, and alpha -adaptin (24, 39). A previous study (20), as well as the present one, showed that Gaf-1/Rip11 binds gamma -tubulin.

Both N-terminal and C-terminal regions of gamma -SNAP contribute to the binding to Gaf-1/Rip11. Interestingly, the corresponding regions of alpha -SNAP are known to interact with SNAREs (9, 40). Because gamma -SNAP does not bind SNAREs, one plausible possibility is that Gaf-1/Rip11 may provide a docking site for gamma -SNAP as SNAREs do for alpha -SNAP. If this were the case, a complex comprising gamma -SNAP and Gaf-1/Rip11 would be disassembled in a manner coupled to NSF-mediated ATP hydrolysis. Our present results clearly showed the requirement of NSF for the disassembly of the gamma -SNAP-Gaf-1/Rip11. It is possible that gamma -SNAP, in cooperation with NSF, may regulate the function of members of the Rab11-interacting protein family.

    ACKNOWLEDGEMENTS

We thank K. Mitsui and K. Okada for technical assistance and Dr. R. Prekeris for critical reading of the manuscript. We also thank Dr. T. Yoshimori at the National Institute for Basic Biology, Dr. Y. Takai at Osaka University, and Dr. S. W. Whiteheart at the University of Kentucky College of Medicine for kindly providing useful materials.

    FOOTNOTES

* This work was supported in part by Grants-in-aid for Scientific Research 13680792, 10215205, and 14380339 from the Ministry of Education, Science, Sports and Culture of Japan, and by ONO Medical Research Foundation.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.

Dagger To whom correspondence should be addressed. Tel.: 81-426-77-7496; Fax: 81-426-76-8866; E-mail: tagaya@ls.toyaku.ac.jp.

Published, JBC Papers in Press, January 27, 2003, DOI 10.1074/jbc.M213205200

    ABBREVIATIONS

The abbreviations used are: NSF, N-ethylmaleimide-sensitive factor; GST, glutathione S-transferase; NEM, N-ethylmaleimide; SNAP, soluble NSF attachment protein; SNARE, SNAP receptor.

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