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Correspondence to Peter Novick: peter.novick{at}yale.edu
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Introduction |
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In S. cerevisiae, the polarized transport of secretory vesicles to the bud tip or, later in the cell cycle, to the mother-bud neck, depends on the actin cytoskeleton and the actin-based myosin motor protein Myo2p (Pruyne et al., 1998; Karpova et al., 2000). An important factor in this transport event is Sec4p, the founding member of the Rab branch of the Ras superfamily of small GTPases (Salminen and Novick, 1987; Goud et al., 1988). Rab proteins are so-called molecular switches, which cycle between an "on" (GTP bound) and "off" (guanosine 5'-diphosphate [GDP] bound) state. This GTPase switch is influenced by guanine nucleotide exchange factors (GEFs), which trigger the binding of GTP, thus activating the Rabs, and GTPase-activating proteins, which accelerate hydrolysis of the bound GTP to GDP, inactivating the GTPase (for review see Pfeffer, 2001; Segev, 2001). Rabs are thought to accomplish their function by binding specific effector proteins in their GTP-bound state (for review see Pfeffer, 2001; Zerial and McBride, 2001).
Sec4p was found in a screen for mutants that block exocytosis and accumulate secretory vesicles at a restrictive temperature (Novick et al., 1980). Mutants of SEC2, the Sec4p GEF, show an accumulation of vesicles randomly distributed throughout the cell, implying that the activation of Sec4p by Sec2p directs the polarized delivery of secretory vesicles (Walch-Solimena et al., 1997). Supporting the view that activated GTP-Sec4p promotes Myo2p-dependent movement of secretory vesicles along actin cables, Sec4p was found to coimmunoprecipitate with Myo2p (Wagner et al., 2002).
Although mutations in SEC4 tightly block secretion (Novick et al., 1980), mutations in actin (ACT1) and MYO2 depolarize secretion and cell surface growth but do not block secretion (Govindan et al., 1995; Karpova et al., 2000). These results imply that Sec4p has at least one function in addition to its role in polarized vesicle delivery. A clue toward one such function came from the identification of Sec15p as a Sec4p effector (Guo et al., 1999b). Sec15p is a subunit of the exocyst, an octameric complex required for tethering secretory vesicles to the plasma membrane in preparation for fusion (TerBush et al., 1996; Guo et al., 1999a). Sec8p, another exocyst subunit, was recently found to coimmunoprecipitate with Sec4p, suggesting that the entire exocyst complex acts downstream of Sec4p (Toikkanen et al., 2003). Furthermore, Sec4p is required for the assembly of the exocyst complex (Guo et al., 1999b).
It has become increasingly clear that Rab GTPases interact with a variety of effectors in order to fulfill their functions in the cell (for review see Zerial and McBride, 2001; Deneka et al., 2003). Combined with the evidence that Sec4p regulates both the transport of secretory vesicles to and fusion with the plasma membrane, it seems likely that there are still more Sec4p effectors to be found. The identification of additional effectors would provide important new insights into the molecular function of Sec4p.
Lethal giant larvae (lgl) was first identified as a tumor suppressor gene in the fly Drosophila melanogaster (for review see Wodarz 2000; Bilder 2004). lgl mutant flies were found to develop malignant tumors in the larval brain and imaginal discs that appear to result from a loss of cell polarity. Subsequently, homologues of lgl have been identified in many organisms, ranging from yeast to humans (for review see Bilder 2004). Because lgl family members are often found to be associated with the actin cytoskeleton, it has been argued that the observed polarity defects in cells bearing lgl mutations are caused by defects in the actin cytoskeleton (Strand et al., 1994; Peng et al., 2000; for review see Baek, 2004). However, data are accumulating that lgl family members function in polarized membrane traffic. D. melanogaster lgl is required for the targeting of proteins to the basolateral membrane (Peng et al., 2000), and the yeast homologues of lgl, Sro7p, and Sro77p (also known as Sop1p and Sop2p, respectively) are redundantly required for exocytosis (Lehman et al., 1999). Sro7p and Sro77p are 55% identical (Kagami et al., 1998; Lehman et al., 1999). Both proteins were originally identified as high-copy suppressors of rho3
(Kagami et al., 1998), a Rho GTPase required for actin cytoskeleton polarity and polarized exocytosis (Matsui and Toh-e, 1992b; Imai et al., 1996; Adamo et al., 1999).
In this study, we describe the identification of Sro7p as an effector of Sec4p. Sro7p from yeast extracts as well as purified Sro7p interact specifically with the GTP-bound form of Sec4p. Sro7p was found to coimmunoprecipitate with Sec4p, demonstrating that the interaction we observed in vitro also occurs in vivo. Moreover, we found that Sro7p, Sec4p, and the t-SNARE Sec9p can form a ternary complex, suggesting that Sec4p regulates SNARE function through Sro7p. In agreement with this, genetic analysis shows that Sro7p shares a function with the exocyst downstream of Sec4p.
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Results |
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S or GDP and, subsequently, incubated with wild-type yeast extract. As a control, GST bound to beads was also incubated with extract. The beads were washed several times, and bound proteins were eluted with high salt (see Sec4p affinity chromatography for details). Despite the presence of background proteins (Fig. 1 C, GST lane), differences could be readily detected between the protein bands in the GST-Sec4p-GTPS and GST-Sec4p-GDP affinity chromatography samples (Fig. 1 C). The protein mixture of each sample was TCA precipitated and subjected to mass spectrometry analysis. Common background proteins were identified by their abundance in both samples and by a survey of published literature (Ho et al., 2002). By definition, an effector binds more strongly to the GTP-bound form of a GTPase than to the GDP-bound form. One measure of the relative abundance of a protein in a protein mixture examined by mass spectrometry is the percentage of residues in the protein sequence that are represented by at least one peptide. We considered all proteins with an at least threefold higher coverage in the sample retrieved from the GTPS-bound versus the GDP-bound form of Sec4p to be potential Sec4p effectors. Among the identified proteins meeting these criteria was Sro7p, a yeast member of the lgl family of proteins.
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S bound compared with its GDP-bound form. To validate these findings, we repeated the affinity chromatography with an extract from yeast cells expressing an integrated HA3-tagged allele of Sro7p. The tag did not interfere with the functionality of the protein, as demonstrated by its ability to suppress the cold sensitivity of an sro7 sro77 double mutant and the salt sensitivity of an sro7 mutant strain (Fig. 2 A and not depicted). Western blot analysis confirmed that Sro7-HA3p migrates at its expected molecular weight (Fig. 2 B). An extract of this strain was incubated with GST-Sec4p in its different nucleotide-bound states or in the nucleotide-free state, GST-Ypt1p and GST. The latter two were used as specificity controls. Ypt1p is another member of the Rab GTPase family that is required for ER-to-Golgi transport in S. cerevisiae (Jedd et al., 1995). To test whether this method indeed distinguishes the different nucleotide-bound states and the nucleotide-free state of Sec4p, we used antibodies to probe for Sec2p and Sec15p. As mentioned above, Sec15p is the only previously documented effector of Sec4p, which was shown by two-hybrid analysis to bind preferentially to a hydrolysis-deficient (GTP locked) allele of Sec4p (Guo et al., 1999b). Sec2p is the exchange factor of Sec4p, which preferentially binds to the nucleotide-free state of Sec4p and, with lesser affinity, to the GDP-bound form of Sec4p (Walch-Solimena et al., 1997; Ortiz et al., 2002). As shown in Fig. 2 C, Sec15p binds specifically to the GTPS-bound form of GST-Sec4p (
-Sec15), whereas Sec2p binds with the highest affinity to the nucleotide-free state of GST-Sec4p (-Sec2), thus confirming the nucleotide specificity of the method. To detect Sro7-HA3p, these samples were analyzed by Western blotting with an -HA antibody. Confirming the result obtained by mass spectrometry, Sro7-HA3p was found to bind much more efficiently to the GTPS-bound form of GST-Sec4p than to its GDP-bound or nucleotide-free state (Fig. 2 C, -HA).
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-HA), establishing the specificity of the Sro7p–Sec4p interaction. Approximately 2–4% of total Sro7-HA3p was found to bind to GTPS-Sec4p in this assay. The amount of Sro7p bound to GTP-Sec4p in this assay exceeds the amount of bound Sec15p (Fig. 2 C, compare -Sec15 with -HA). Interestingly, the same amount of Sro7-HA3p binds to GTPS-Sec4p when only half the amount of extract is used (not depicted), suggesting that the amount of activated Sec4p available for Sro7p binding is limiting in this assay. Altogether, our data indicate that Sro7p from yeast extract binds preferentially to the GTP-bound form of Sec4p, confirming the result obtained by mass spectrometry.
Sro7p binds directly to Sec4p
We next determined whether purified Sro7p and Sec4p bind to each other in the absence of other proteins. Because Sro7p cannot be purified from bacteria (unpublished data), it was purified from yeast using a multistep procedure (see Purification of full-length Sec9 and Sro7 for details). This purification resulted in an Sro7p preparation that appears homogeneous by SDS-PAGE and Coomassie staining (Fig. 3 A) and dissociated from its binding protein, Sec9p (Lehman et al., 1999; unpublished data). As shown in Fig. 3 B, purified Sro7p binds to GST-Sec4p preferentially in the presence of GTPS. The amount of Sro7p bound to GST-Sec4p ranges from 
5 to 20% of total Sro7p bound to GTPS-Sec4p, and 1/20–1/10 of this amount bound to the GDP-bound or nucleotide-free Sec4p (Fig. 3 B). The observed binding is specific because Sro7p does not bind to any of the nucleotide-bound and -free forms of GST-Ypt1 or GST alone (Fig. 3 B and not depicted). Thus, purified Sro7p binds to Sec4p in its activated state. Given the strength of the observed interaction (Fig. 3 B) and the purity of Sro7p (Fig. 3 A), we conclude that this interaction is very likely to be direct because any copurifying factor would be substoichiometric.
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-HA antibody, and coimmunoprecipitating Sro7p was detected by Western blotting with an -Sro7p antibody. As shown in Fig. 4, Sro7p coimmunoprecipitates with HA-Sec4p. This interaction is specific because (1) only a background amount of Sro7p is found to interact with Ypt1p; (2) the signal requires the cooverexpression of both Sec4p and Sro7p; and (3) no signal can be detected when the antibody is omitted from the precipitation reaction (Fig. 4). These data further support the conclusion that Sro7p binds directly to Sec4p because no third protein was overexpressed. Quantification of the interaction revealed that 2% of total Sro7p bound to GST-Sec4p (immunoprecipitated amount set to 100%). This relatively low amount might reflect the predominantly inactivated state of Sec4p in a yeast lysate. Together, our in vivo and in vitro data establish Sro7p as an effector of Sec4p.
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S and Sro7p. Under the conditions used in this assay, 5–10% of the input Sro7p binds to Sec4p. Only background binding of Sec9p to GTPS-Sec4p was observed when Sro7p was omitted from the binding assay, suggesting that Sec9p binds to Sec4p through Sro7p and implying that Sec4p and Sec9p use different binding sites on Sro7p (Fig. 5). The specificity of this interaction was demonstrated by the fact that no significant binding of Sro7p or Sec9p to GDP-Sec4p or GST was detected (Fig. 5, GST). Therefore, our data imply that GTP-Sec4p, Sro7p, and Sec9p are able to form a ternary complex.
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mutant. In agreement with this, it has recently been published that the overexpression of SRO7 rescues the exocytosis defect of the sec3 mutant (Zhang et al., 2005). Interestingly, however, the level of suppression achieved by overexpression of SRO7 is not as strong as that achieved by 2µ SEC4 (Fig. 6 A, compare sec3 2µ SRO7 with sec3 2µ SEC4). We found that the deletion of SEC3 increases the doubling time of a yeast strain about twofold compared with wild-type yeast at 30°C in synthetic complete (SC) minimal medium (225 ± 21 min vs. 125 ± 7 min; Fig. 6 B). Overexpression of SEC4 rescues this growth defect to nearly wild-type levels (145 ± 7 min), but sec3 cells overexpressing SRO7 still display a strong growth defect (190 ± 14 min; Fig. 6 B). Similarly, 2µ SRO7 does not suppress the lethality of sec3 on yeast peptone dextrose (YPD) media (Fig. 6 C; Wiederkehr et al., 2003). One interpretation of these data is that Sec4p signals to other effectors in addition to Sro7p and the exocyst to achieve vesicle fusion. In support of our suggestion of converging functions for Sro7p and the exocyst, deletion of SRO7 in a sec3 strain further aggravates its growth defect (Fig. 7 A). We observed that the doubling time of a sec3 sro7 strain (360 ± 28 min) is almost twice that of a sec3 single mutant strain (225 ± 21 min; Fig. 7 B). This growth phenotype is accompanied by a significant drop in exocytosis in the sec3 sro7 mutant of 10% compared with the sec3 mutant (73 ± 7% vs. 60 ± 5% of secreted invertase; Fig. 7 C). This further implicates Sro7p and the exocyst in interrelated functions on the exocytic pathway.
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sro7 mutant strain, we decided to test whether the deletion of SRO7 would have a similar influence on the growth of other exocyst mutant strains. For that purpose, we used a collection of temperature-sensitive late secretory mutant strains (sec1-1, sec2-41, sec3-2, sec4-8, sec5-24, sec6-4, sec8-9, sec9-4, sec10-2, and sec15-1). We observed that sec2-41, sec3-2, sec4-8, sec8-9, sec9-4, and sec15-1 in combination with sro7 displayed slower growth compared with the single mutant strains at the permissive temperature of 24°C (Fig. S1, available at http://www.jcb.org/cgi/content/full/jcb.200510016/DC1). Interestingly, the most striking feature we observed is that combining a deletion of SRO7 with almost all of the heat-sensitive mutants lead to a synthetic growth defect at 14°C (Table II and Fig. S1). Double deletion of SRO7 and its paralogue SRO77 has been found to lead to cold sensitivity of the resulting double mutant strain (Kagami et al., 1998; Lehman et al., 1999), which demonstrated that their gene products share a common function. We found that the double mutants of the Rab GTPase Sec4p (sec4-8) or its GEF Sec2p (sec2-41) with sro7 display synthetic lethality at 14°C (Table II and Fig. S1). This result further indicates a common function of Sro7p and Sec4p. The fact that sro7 causes sec1-1, a heat-sensitive mutant of the SNARE-interacting protein Sec1p, and sec9-4, a mutant of the t-SNARE Sec9p, to become cold sensitive (Table II and Fig. S1) adds genetic evidence for a role of Sro7p in SNARE function in yeast. Interestingly, we also found that the deletion of SRO7 leads to cold sensitivity in only a subset of the temperature-sensitive exocyst mutant strains (Table II and Fig. S1). These data might either reflect the relative strength of these mutant alleles at low temperature or indicate that only those subunits share a function with Sro7p and, therefore, add further evidence for a functional specialization of exocyst subunits within the complex (Wiederkehr et al., 2004). Altogether, our genetic data support a possible role for Sro7p in transferring the signal of the Rab GTPase Sec4p to SNARE function in yeast.
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mutant strain, we hypothesized that 2µ SRO7 might also be able to overcome the lethality of exo70 and sec5 mutant strains. As shown in Fig. 8, overexpression of SRO7 on a 2µ plasmid indeed rescues the lethality of both exo70 (Fig. 8 A) and sec5 (Fig. 8 B) mutant strains. Because we found that Sro7p is an effector of Sec4p with an exocyst-related function, it appeared likely that Sro7p would be required for the Sec4p-mediated rescue of exo70 and sec5 mutant strains (Wiederkehr et al., 2004). Indeed, the deletion of SRO7 reduces the growth of both exo70 and sec5 strains rescued by the overexpression of SEC4 from a 2µ plasmid (Fig. 9, A and B; compare exo70 2µ SEC4 or sec5 2µ SEC4 with exo70 sro7 2µ SEC4 or sec5 sro7 2µ SEC4). We found that the doubling times of the exo70 sro7 2µ SEC4 (240 ± 21 min) or sec5 sro7 2µ SEC4 (242 ± 31 min) yeast strains are significantly increased compared with the yeast strains without additional deletion of SRO7 (190 ± 14 min and 185 ± 21 min, respectively; Fig. 9, C and D). In striking contrast, deletion of SRO7 was found to only have minor influences on the growth of both exo70 and sec5 mutant strains rescued by overexpression of SEC1 from a 2µ plasmid on either solid or liquid media (Fig. 9, compare exo70 2µ SEC1 or sec5 2µ SEC1 with exo70 sro7 2µ SEC1 or sec5 sro7 2µ SEC1). Therefore, these data provide genetic evidence that Sro7p functions downstream of Sec4p in an exocyst-related function. They further imply that although Sec4p signaling is upstream of Sro7p and the exocyst, Sec1p functions downstream of both (summarized in the model in Fig. 10). Our results are also consistent with previous data that showed that Sec4p and Sec1p use different mechanisms for suppression of exocyst deletion mutations (Wiederkehr et al., 2004).
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strain. Sec15p is the subunit of the exocyst that directly interacts with Sec4p (Guo et al., 1999b). It has been previously shown that the overexpression of SEC4 and SRO7 was able to suppress the temperature sensitivity of a sec15-1 mutant strain (Fig. S2 A, available at http://www.jcb.org/cgi/content/full/jcb.200510016/DC1; Salminen and Novick, 1987; Guo et al., 1999b; Lehman et al., 1999). However, under all tested conditions (different media and temperatures), neither 2µ SRO7 nor 2µ SRO7 in combination with 2µ SEC4 were able to suppress the lethality of a sec15 strain (Fig. S2 B and not depicted). These genetic data indicate that Sro7p shares some, but not all, functions with the exocyst in yeast. |
Discussion |
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Several previously published reports support our findings. Sro7p and its paralogue Sro77p were originally identified as high-copy suppressors of Rho3p (Matsui and Toh-e, 1992a; Kagami et al., 1998), which is a Rho GTPase required for actin cytoskeleton polarity and polarized exocytosis in yeast (Matsui and Toh-e, 1992b; Imai et al., 1996; Adamo et al., 1999). Another protein found in this screen (Sro6p) was subsequently identified as Sec4p. These genetic data suggest that the identified proteins positively influence cell polarity and/or polarized exocytosis, as had been shown for Sec4p (Salminen and Novick, 1987; Goud et al., 1988). Subsequently, Sro7/77p have also been found to be required for exocytosis in yeast (Lehman et al., 1999). Additionally, the overexpression of Sro7p was found to suppress the cold sensitivity of a sec4-P48 mutant (Brennwald et al., 1994), which suggested that Sro7p might act downstream of Sec4p function.
Sro7p genetically interacts with the exocyst downstream of Sec4p
Genetic data presented in this study indicate that the function of Sro7p partially overlaps with that of the exocyst (Figs. 6– 9), an eight-subunit vesicle-tethering complex required for tethering secretory vesicles to the plasma membrane (TerBush et al., 1996; Guo et al., 1999a). We found that the overexpression of SRO7 suppresses the growth defects of three different exocyst deletion mutants (sec3, sec5, and exo70; Figs. 6 and 8), extending recently published data (Zhang et al., 2005). We also showed that the deletion of SRO7 impairs the growth and secretory function of a sec3 strain (Fig. 7), which further implies that Sro7p and the exocyst function in concert.
We recently established that the overexpression of either Sec4p or Sec1p can bypass the inviability of sec5 or exo70 strains (Wiederkehr et al., 2004). Interestingly, we now demonstrate that the deletion of SRO7 in exo70 or sec5 strains reduces growth only when SEC4 is overexpressed (Fig. 9). If SEC1 is overexpressed, no significant difference in growth can be detected upon SRO7 deletion (Fig. 9). These data provide genetic evidence that Sro7p acts downstream of Sec4p in its capacity as a suppressor and demonstrate that Sro7p is involved in a Sec4p- and exocyst-related function (Fig. 10). Moreover, they further strengthen the findings by Wiederkehr et al. (2004) that indicate that Sec4p and Sec1p use different mechanisms in their suppression of the two exocyst mutants.
Although SRO7, SEC1, and SEC4 can each act as a high-copy suppressor of sec3, sec5, and exo70, there is no simple hierarchy in the efficiency of suppression. Thus, SEC4 suppresses sec3 and sec5 better than does SRO7 (Figs. 6 and 8), but SRO7 is somewhat better at suppressing exo70 than is SEC4 (Fig. 8). Furthermore, SEC1 suppresses exo70 much better than does SEC4, but SEC4 suppresses sec5 much better than does SEC1 (Fig. 8). Although this pattern is presently difficult to interpret, it does support the notion that different subunits of the exocyst fulfill distinct functions (Wiederkehr et al., 2004), possibly in tethering and regulation of SNARE function.
As mentioned above, the Sec15p subunit of the yeast exocyst is also a Sec4p effector (Guo et al., 1999b). If Sro7p and the exocyst have purely redundant functions downstream of Sec4p, the overexpression of one effector should overcome the loss of the other. Contrary to this prediction, we found that overexpression of SRO7, either alone or in combination with SEC4, did not suppress the lethality of a sec15 mutant under all conditions tested (Fig. S2 B and not depicted). Thus, these data indicate that Sro7p and the exocyst have interrelated but not identical functions. In agreement with this, the overexpression of individual exocyst subunits did not suppress the salt sensitivity of the sro7 mutant (Fig. S3, available at http://www.jcb.org/cgi/content/full/jcb.200510016/DC1) or the cold sensitivity of an sro7 sro77 mutant (Zhang et al., 2005). Although it might simply be that more than one subunit (i.e., a subcomplex) is required for suppression, another explanation for this finding is that Sro7p and Sro77p have important cellular functions beyond their role in exocytosis. In agreement with this, overexpression of either of the t-SNAREs, SEC9 and SSO1, or the SNARE regulator SEC1 failed to suppress the sro7 sro77 phenotype (Zhang et al., 2005). Sro7/77p have been shown to interact biochemically with the yeast type II myosin Myo1p, an interaction that appears to play a role in the remodeling of the actin cytoskeleton (Kagami et al., 1998), which is consistent with data concerning lgl family members from other organisms (see Introduction). Another explanation for the failure of overexpression of single exocyst subunits to suppress the salt or cold sensitivity of Sro7/77p mutants could be that Sro7p and Sro77p act downstream of some, but not all, aspects of exocyst function (Wiederkehr et al., 2004; Zhang et al., 2005).
Sro7p links a Rab (Sec4p) to a t-SNARE (Sec9p)
Rab GTPase activity has previously been implicated in the regulation of SNARE complex assembly (Lian et al., 1994; Sogaard et al., 1994). Furthermore, genetic evidence suggested that plasma membrane SNAREs act in response to Rabs because the overexpression of SEC9 has been found to suppress the growth defect of a sec4-P48 mutant strain (Brennwald et al., 1994). Nonetheless, a direct interaction of activated Sec4p and the exocytic SNAREs could not be detected (Grote and Novick, 1999). We provide evidence in this study that GTP-bound Sec4p interacts with the plasma membrane SNAREs via Sro7p. The Sec4p effector Sro7p was found to interact with the t-SNARE Sec9p (Lehman et al., 1999), and recent data indicate that this interaction is important for Sro7p's function in secretion (Gangar et al., 2005). We have demonstrated that Sec9p can associate with Sec4p, but only in the presence of GTPS and Sro7p (Fig. 5). This interaction provides a link between Rab signaling and SNARE function in yeast exocytosis.
Together, two convergent signaling pathways from the Rab GTPase Sec4p appear to lead to vesicle fusion in yeast (Fig. 10). Secretory vesicles carrying activated Sec4p transmit a signal to Sec15p, which leads to exocyst assembly and vesicle tethering (Guo et al., 1999b). A recently documented association of Sec1p with the exocyst (Wiederkehr et al., 2004) potentially links this pathway to SNARE function. In a second branch of the pathway, Sec4p transmits a signal through the lgl family member Sro7p. Because Sec4p, Sro7p, and the t-SNARE Sec9p can assemble into a ternary complex, we propose that Sro7p conveys the signal from the Rab GTPase to SNARE function in yeast. These interactions may normally occur after vesicle tethering by the exocyst. There appears to be crosstalk between these two pathways because Sro7p has recently been shown to associate with the exocyst subunit Exo84p (Zhang et al., 2005). Further studies will be necessary to explore these proposals.
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Materials and methods |
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0.3, and 10-fold dilutions were spotted onto YPD media or SC plates and incubated at the indicated temperatures for 2–3 (25°C and above) or 7–8 (14°C) d.
Plasmids
Standard techniques were used for plasmid construction. The SEC4 ORF was amplified by PCR from genomic DNA and subsequently inserted into plasmid pGEX5X-1 (GE Healthcare) to create the GST-SEC4 expression vector (pNB 1245). The plasmid carrying GST-YPT1 was described previously (Wang et al., 2000).
The plasmid carrying SRO7 behind the GAL1 promoter (pNB 1246) was created by inserting the SRO7 ORF into plasmid pNB 530 (GAL1 promoter, ADH1 terminator, and URA3 marker). The plasmids carrying HA-SEC4 (pNB 833) and HA-YPT1 (pNB 829) behind the GAL1 promoter and the control plasmid pNB 529 have been described previously (Grote and Novick, 1999).
Plasmid pB 745 (2µ SRO7::URA3) was described previously (Lehman et al., 1999). 2µ plasmids pNB 142, 680, 807, 690, 216, 328, 685, 148, 887, and 888 were used to overexpress SEC4, SEC1, SEC3, SEC5, SEC6, SEC8, SEC10, SEC15, EXO70, or EXO84, respectively (P. Novick collection).
Antibodies
The -Sro7p antibody was described previously (Lehman et al., 1999). Clones 3F10 (rat monoclonal; Roche) and 16B12 (mouse monoclonal; Convance) were used as antibodies against the HA epitope. Rabbit polyclonal antibodies were used for the detection of Sec2p or Sec15p (P. Novick collection). A goat -GST antibody (Sigma-Aldrich) was used to detect GST fusion proteins.
Yeast extract for Sec4p affinity chromatography
27 liters of wild-type yeast culture were lysed by homogenization in a microfluidizer (Microfluidics Corporation) in 140 ml of nucleotide-binding (NB) buffer (20 mM Hepes, pH 7.2, 100 mM KCl, 5 mM MgCl2, and 1 mM DTT) containing 1 mM PMSF, 5 µg/ml pepstatin A, and complete protease inhibitor EDTA-free cocktail (Roche). Triton X-100 was added to 1%, and unbroken cells and debris were eliminated by centrifugation at 10,000 g for 25 min at 4°C. The extract was dialyzed against NB buffer overnight. The concentration of the extract was adjusted to 40 mg/ml.
Purification of GST-Sec4, GST-Ypt1, and GST and nucleotide exchange
GST fusion proteins were purified from BL21 Escherichia coli strains (Novagen) as described previously (Christoforidis and Zerial, 2000; Wang et al., 2000; Idrissi et al., 2002). For nucleotide loading, GST-Sec4p or GST-Ypt1p were incubated with a 200-fold excess of either GTPS or GDP in NB for 2 h at 30–37°C. To obtain the nucleotide-free state, the proteins were incubated in NB buffer supplemented with 10 mM EDTA.
Purification of full-length Sec9 and Sro7
Full-length Sec9p tagged with COOH-terminal His6 tag was purified from E. coli as described previously (Gangar et al., 2005). Sro7p with an NH2-terminal protein A/tobacco etch virus (TEV) tag was isolated from lysates prepared from overexpressing yeast strains using affinity chromatography with IgG Sepharose beads. It was then eluted by cleavage of the protein A tag with TEV protease and subsequently purified by ion exchange chromatography to apparent homogeneity based on SDS-PAGE analysis.
Sec4p affinity chromatography
The protocol was adapted from Christoforidis and Zerial (2000). In brief, 100 µl GTPS- or GDP-bound GST-Sec4p or GST-containing beads (750 µg of protein) were incubated with 25 ml of wild-type yeast extract (40 mg/ml) for 2 h at 4°C. After several washings, bound proteins were eluted with elution buffer (20 mM Hepes, pH 7.2, 1.5 M NaCl, 20 mM EDTA, and 1 mM DTT) supplemented with 5 mM of the opposing nucleotide. The proteins were TCA precipitated, dried, and analyzed by mass spectrometry.
For the experiment in Fig. 2, 2.5 µl of loaded beads (15 µg) were incubated with 1 ml of a 20-mg/ml yeast extract (lysed using a French press; Sim-Amico Spectronic Instruments). Bound proteins were analyzed by Western blotting.
Mass spectrometry
Samples were suspended in 8 M urea and 100 mM Tris, pH 8.5, reduced with 100 mM TCEP, and cysteines were alkylated with 55 mM iodoacetamide. Lys-C was used to digest the proteins for 4 h at 37°C at a concentration of 1 µg/100 µl. CaCl2 was added to ensure tryptic specificity at 1 mM, and trypsin was used to digest the samples further at 1 µg/100 µl. The digests were then analyzed by µLC/µLC-MS/MS using an ion trap mass spectrometer (LCQ Deca; ThermoElectron). Multidimensional chromatography was performed online according to MacCoss et al. (2002) using the following salt steps of 500 mM ammonium acetate: 10, 25, 35, 50, 65, 80, and 100%. Tandem mass spectra were collected in a data-dependent fashion by collecting one full MS scan (m/z range = 400–1,600) followed by MS/MS spectra of the three most abundant precursor ions. The collection of resulting spectra was then searched against a database of yeast ORFs obtained from the Saccharomyces genome database (release date 08/27/04) using the SEQUEST algorithm (Eng et al., 1994). Peptide identifications were organized and filtered using the DTASelect program (Tabb et al., 2002). Filtering criteria for positive protein identifications in the Smt3p purification were the identification of two unique, fully tryptic peptides with Xcorr values >2.0 for +1 spectra, 2.2 for +2 spectra, and 3.75 for +3 spectra.
In vitro binding assays
Glutathione beads carrying 6 µM GST-Sec4p or GST were washed with 20 mM Tris, pH 7.5, 100 mM NaCl, and 1 mM DTT and were incubated in 20 mM Tris, pH 7.5, 100 mM NaCl, 5 mM EDTA, and 1 mM DTT in the presence of either 100 µM GTPS, 100 µM GDP, or no nucleotide for 15 min at 25°C. Then, MgCl2 was added to a final concentration of 25 mM and incubated 45 min at 25°C. Binding assays were performed in binding buffer (20 mM Tris-HCl, pH 7.4, 140 mM NaCl, 5 mM MgCl2, 1 mM DTT, and 0.5% Triton X-100). The final concentrations of GST/GST-Sec4p in the binding reactions were 4 µM, whereas concentrations of Sro7p or Sec9p were 1 µM. Samples were incubated at 4°C for 1 h. The beads were washed four times with binding buffer, and bound proteins were subjected to Western blot analysis. Sro7p and Sec9p were detected with rabbit -Sro7 or -Sec9 antibodies and -rabbit IgG conjugated to AlexaFluor680 and were analyzed on an Odyssey Infrared Imaging System (LI-COR). For the experiment in Fig. 5, Sro7p–Sec9p mixtures (or Sro7p or Sec9p alone) were preincubated on ice for 1 h to allow the formation of binary complexes before their addition to the coated glutathione beads.
Immunoprecipitation
Yeast strains 2,592–2,595 were grown overnight in yeast peptone media containing raffinose at 25°C to an OD600 of 0.4. Production of HA-Sec4p, HA-Ypt1p, and Sro7p was then induced by the addition of 2% galactose for 45 min. Cell pellets were resuspended in immunoprecipitation buffer (20 mM Hepes, pH 7.2, 150 mM KCl, 1 mM DTT, 6 mM MgCl2, and 1 mM EDTA) containing 1 mM GTP, 1% NP-40, and protease inhibitors (1 mM PMSF, 2 µg/ml pepstatin A, 2 µg/ml chymostatin, 2 µg/ml aprotinin, 2 µg/ml leupeptin, and 2 µg/ml antipain). 2 g zirconia-silica beads were added, and the cells were lysed by homogenization in a Mini-Bead Beater (Biospec Products). Unbroken cells and debris were eliminated by centrifugation at 10,000 g for 20 min at 4°C. The concentration of the yeast extracts was adjusted to 1 mg/ml, 30 µl of 50% protein G–Sepharose beads were added to 500 µl of extract, and the reaction was incubated for 90 min at 4°C. Beads were pelleted, 7.5 µl rat -HA antibody was added to the supernatants, and the reactions were incubated overnight at 4°C. 6 µl of 50% protein G–Sepharose beads were added and incubated for another 30 min. The beads were pelleted, washed several times with immunoprecipitation buffer, and bound proteins were subjected to Western blot analysis.
Invertase secretion
The monitoring of invertase secretion was performed as described previously (Wiederkehr et al., 2003).
Image analysis
Data were digitalized using a scanner (HP Scanjet 4570c; Hewlett Packard).
Online supplemental material
Fig. S1 shows the growth of exocytic temperature-sensitive mutants combined with the deletion of SRO7 compared with the single mutants and wild-type yeast at 24 and 14°C (data are summarized in Table II). Fig. S2 shows that the overexpression of SEC4 and SRO7 suppresses the growth phenotype of a sec15-1 mutant strain (A) but not the deletion of SEC15 (B). Fig. S3 shows that the overexpression of single exocyst subunits does not suppress the salt sensitivity of an sro7 strain.
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Acknowledgments |
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This work was supported by grants from the National Institutes of Health to P. Novick (GM 35370 and CA 46128), J. Yates III (P41 RR11823-10), and P. Brennwald (R01GM54712).
Submitted: 4 October 2005
Accepted: 22 November 2005
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