Cyclical Regulation of the Exocyst and Cell Polarity Determinants for Polarized Cell Growth

Allison Zajac^*, Xiaoli Sun^*, Jian Zhang, and Wei Guo

Department of Biology, University of Pennsylvania, Philadelphia, PA 19104-6018

Submitted October 14, 2004; Revised November 26, 2004; Accepted December 28, 2004
Monitoring Editor: Keith Mostov

ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Polarized exocytosis is important for morphogenesis and cellgrowth. The exocyst is a multiprotein complex implicated intethering secretory vesicles at specific sites of the plasmamembrane for exocytosis. In the budding yeast, the exocyst islocalized to sites of bud emergence or the tips of small daughtercells, where it mediates secretion and cell surface expansion.To understand how exocytosis is spatially controlled, we systematicallyanalyzed the localization of Sec15p, a member of the exocystcomplex and downstream effector of the rab protein Sec4p, invarious mutants. We found that the polarized localization ofSec15p relies on functional upstream membrane traffic, activatedrab protein Sec4p, and its guanine exchange factor Sec2p. Theinitial targeting of both Sec4p and Sec15p to the bud tip dependson polarized actin cable. However, different recycling mechanismsfor rab and Sec15p may account for the different kinetics ofpolarization for these two proteins. We also found that Sec3pand Sec15p, though both members of the exocyst complex, relyon distinctive targeting mechanisms for their localization.The assembly of the exocyst may integrate various cellular signalsto ensure that exocytosis is tightly controlled. Key regulatorsof cell polarity such as Cdc42p are important for the recruitmentof the exocyst to the budding site. Conversely, we found thatthe proper localization of these cell polarity regulators themselvesalso requires a functional exocytosis pathway. We further reportthat Bem1p, a protein essential for the recruitment of signalingmolecules for the establishment of cell polarity, interactswith the exocyst complex. We propose that a cyclical regulatorynetwork contributes to the establishment and maintenance ofpolarized cell growth in yeast.

INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Exocytosis is a basic membrane traffic event mediated by transport,docking, and fusion of secretory vesicles carrying proteinsand lipids to defined areas of the plasma membrane. For mosteukaryotic cells, exocytosis is spatially controlled by signalingmolecules and the cytoskeleton. On the other hand, polarizedexocytosis is important for the delivery of polarity regulators.The simple eukaryote Saccharomyces cerevisiae grows asymmetricallyby "budding," a seemingly simple process that requires sophisticatedmechanisms that couple exocytosis to cell polarization and cellcycle progression. At the early stages of the cell cycle, polarizeddelivery of lipid and membrane proteins to the bud is importantfor daughter cell growth. In addition, the polarized secretionof cell surface glucanases is needed to modify the rigid yeastcell wall so that the specific areas of the daughter cell surfacecan expand. The distinctive growth characteristics, in combinationwith the facile genetics and well-studied genomics, make thebudding yeast an excellent model system to study spatial regulationof exocytosis.

The late stage of exocytosis in yeast consists of at least threesteps. First, post-Golgi secretory vesicles are targeted todesignated areas of plasma membrane via actin cables. The classV myosin, Myo2p, serves as a motor for this transport process(Govindan et al., 1995; Pruyne et al., 1998; Schott et al.,1999; Karpova et al., 2000). Second, the vesicles are tetheredto specific plasma membrane domains mediated by a multiproteincomplex, the exocyst (Guo et al., 2000; Whyte and Munro, 2002;Hsu et al., 2004; Chu and Guo, 2004). Finally, interactionsbetween vesicle and plasma membrane integral membrane proteins,termed v-SNAREs and t-SNAREs, respectively (SNARE, soluble N-ethylmaleimide-sensitivefusion attachment protein receptors), lead to the fusion ofthe bilayers of the secretory vesicle and the plasma membrane(Rothman, 1994). This fusion event allows the secretion of vesiclecontents and the incorporation of membrane proteins at specificplasma membrane domains. The rab family of small GTPases aremaster regulators of exocytosis (Novick and Zerial, 1997; Lazaret al., 1997).

The exocyst is an evolutionarily conserved multiprotein compleximplicated in tethering secretory vesicles at specific sitesof the plasma membrane preceding SNARE assembly and membranefusion (Novick and Guo, 2002; Lipschutz and Mostov, 2002; Hsuet al., 2004). It consists of 8 components: Sec3p, Sec5p, Sec6p,Sec8p, Sec10p, Sec15p, Exo70p, and Exo84p. All are hydrophilicproteins that exist in the cytosol and associate with the plasmamembrane (TerBush and Novick, 1995; TerBush et al., 1996; Guoet al., 1999a). In budding yeast, the exocyst proteins are specificallylocalized to regions of active exocytosis and cell surface expansion:the sites of bud emergence, the tips of small daughter cells,and the mother/daughter junction of dividing cells (TerBushand Novick, 1996; Finger et al., 1998; Guo et al., 1999b). Thispattern of localization is in contrast to that of the t-SNAREproteins, which are evenly distributed along the entire yeastplasma membrane (Brenn-wald et al., 1994).

One component of the exocyst complex, Sec3p, is localized tosites of exocytosis independent of ongoing secretion and theactin cytoskeleton (Finger et al., 1998). In a variety of secretionmutants blocked at or before the Golgi apparatus, Sec3-GFP isstill localized at bud tips and mother/daughter cell connections.Furthermore, the localization of Sec3p appears to be independentof the other subunits of the exocyst. Based on these observations,it was proposed that Sec3p represents a spatial landmark forpolarized secretion (Finger et al., 1998). Recent studies demonstratedthat Sec3p directly interacts with Rho1p and Cdc42p, membersof the Rho family of small GTPases through its N-terminus (Guoet al., 2001; Zhang et al., 2001). Cdc42p and Rho1p competefor their binding to this region and disruption of the bindingresults in mislocalization of Sec3p (Guo et al., 2001; Zhanget al., 2001).

While Sec3p is thought to be the exocyst subunit most proximalto the plasma membrane, another subunit, Sec15p, directly interactswith the GTP-bound form of the rab protein, Sec4p, on the secretoryvesicles (Guo et al., 1999b). This interaction is specific forSec4p but not for other rab proteins such as Ypt1p and Ypt51p.Replacement of four amino acids in the "effector loop" of Sec4pwith the corresponding residues of Ypt1p completely abolishedthe interaction of the Rab protein with Sec15p. Sec4p promotesthe protein-protein interactions among the exocyst components,which eventually link Sec15p to Sec3p at the target membrane(Guo et al. 1999a).

To better understand how exocytosis is spatially controlled,we have systematically examined the localization of the exocystin yeast cells. Here we focus on Sec15p, the direct downstreameffector of Sec4p (Guo et al., 1999b). We found that upstreamtraffic and the rab GTPase controls the localization of Sec15pto site of secretion. The targeting of Sec15p is also underthe control of cell polarity determinants and requires polarizedactin cables. Sec3p and Sec15p, though both members of the exocystcomplex, are spatially controlled by different mechanisms. Inaddition to examining how the exocyst is controlled by polarityregulators, we also examined the role of exocytosis on cellpolarity by using different alleles of the secretory mutants.We found that the proper localization of these cell polarityregulators themselves also requires a functional exocytosispathway. We further report that Bem1p, a protein essential forthe establishment of cell polarity, interacts with the exocyst.We propose that a cyclical regulatory mechanism may contributeto the establishment of cell polarity and maintenance of polarizedcell growth in yeast.

MATERIALS AND METHODS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Strains and Growth Conditions
The genotypes of the yeast strains used in this study are listedin Table 1. Standard culture media and genetic techniques wereused (Guthrie and Fink, 1991).

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Table 1. Parental strains used in this study

Observation of GFP-tagged Proteins in Yeast Cells
C-terminal GFP tagging of the exocyst components and Bem1p attheir chromosomes in wild-type and mutant yeast strains wasperformed as previously described (Finger et al., 1998; Guoet al., 1999a). Cells were grown to early log phase in SCD media(synthetic complete plus 2% dextrose) lacking uracil. Yeastcells were fixed as follows: cells were pelleted 1 min at 4°Cat 3000 rpm in an Eppendorf 5415R bench top centrifuge, washedonce in ice-cold phosphate-buffered saline (PBS), and then fixedat 4°C for 10 min in -20°C methanol. The cells werewashed once in -20°C acetone and rehydrated by three washesin PBS for viewing. GFP was scored as mislocalized when it appeareddiffused or in patches in the mother cells. Protein localizationin yeast released from G₀ was examined as previously described(Ayscough et al., 1997).

Immunofluorescence
Immunofluorescence staining of yeast cells was performed aspreviously described (Walch-Solimena et al., 1997). Briefly,the cells were fixed and transferred to isotonic media containing0.1 M KPi, pH 7.4, and 1.2 M sorbitol. After cell wall removalby zymolase, the spheroplasts were attached to eight-well microslidesand then treated with 0.5% SDS in 0.1 M KPi, pH 7.4, and 1.2M sorbitol for 5 min. The cells were then washed 10 times with20 µl per well of PBS containing 1 mg/ml bovine serumalbumin, and nonspecific binding was blocked for 30 min in thesame buffer. The incubation with primary antibodies was performedat room temperature for 2 h. After 10 washes in PBS-bovine serumalbumin buffer, the cells were incubated for 1 h with Alexa-fluor594 secondary antibody. The wells were washed with PBS-bovineserum albumin buffer and then mounted for observation. The immunofluorescencewas visualized with a microscope equipped with epifluorescenceusing a 100x objective. The anti-Sec4p polyclonal antibody wasused at 1:1000 dilution. Immunostaining of myc-tagged Bem1pwas performed with a mouse anti-myc monoclonal antibody (9E10)at 1:500 dilution.

Coprecipitation Assays
The in vivo interaction between Sec15p and Bem1p was performedusing coprecipitation assays. Yeast cells expressing GST orGST-Bem1p in a CEN plasmid under the TEF promoter were grownto early log phase, and cell lysates were prepared by disruptingthe cell wall using glass beads in the lysis buffer (20 mM HEPES-NaOH,pH 7.5, 100 mM NaCl, 1 mM EDTA, 1 mM dithiothreitol, 1% Sigmaprotease inhibitor cocktail). The lysates were incubated withglutathione Sepharose 4B for 1 h at 4°C. The Sepharose werewashed five times and the proteins were separated using 10%SDS-PAGE. Proteins coprecipitated with the GST fusion proteinsfrom the lysates were analyzed by Western blot.

RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Sec15p Polarization Is Dependent on Upstream Traffic and Active Sec4p
Sec15p was previously shown to interact with the GTP-bound formof the rab protein Sec4p. Furthermore, biochemical analysissuggests that the assembly of the exocyst complex is defectivein the sec4 mutant (Guo et al., 1999b). It is possible thatSec15p travels to sites of polarized secretion on vesicles andSec4p regulates this process. If so, mutations affecting theactivity of Sec4p would block the ability of Sec15p to polarizein yeast cells. In addition, defects in upstream trafficking(e.g., ER to Golgi, intra-Golgi transport, etc.) will also affectSec15p delivery as the flow of membranes is blocked. To testthis hypothesis, we examined the localization of Sec15-GFP invarious mutants. These include sec18-1 (defective in SNARE disassemblyand ER-to-Golgi traffic), sec22-3 (defective in ER-to-Golgitraffic), sec7-1 (defective in Golgi traffic), sec4-8 (mutationin the rab protein responsible for post-Golgi exocytosis; Novicket al., 1980). In addition, to further test whether the activatedform of Sec4p is required, we examined the localization of Sec15-GFPin the sec2-59 strain, in which the guanine nucleotide exchangefactor (GEF) of Sec4p is mutated (Walch-Solimena et al., 1997).The yeast cells were grown to early log phase and then shiftedto the restrictive temperature for periods of 10 and 90 min.Cells were then fixed in methanol/acetone and examined for Sec15-GFPlocalization. In wild-type cells, Sec15-GFP was concentratedas a crescent at the bud tip at 25°C, 10 min at 34°C,and 90 min at 34°C (Figure 1A). In contrast, in the mutantcells defective in various stages of traffic or defective inSec4p, Sec15-GFP signals were diffused from the bud after 10min at 34°C. At 90 min, Sec15p remained mislocalized inthese cells. A quantification of the observation is presentedin Figure 1B.

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Figure 1. Sec15-GFP polarization is dependent on upstream traffic and functional Sec4p. (A) Sec15-GFP was expressed in wild-type, sec18-1 (defective in SNARE disassembly and ER-to-Golgi traffic), sec22-3 (defective in ER-to-Golgi traffic), sec7-1 (defective in Golgi traffic), sec4-8 (mutation in the post-Golgi rab protein), and sec2-59 (a mutant allele of the GEF for Sec4p). Cells were grown in SC-Ura media at 25°C to log phase and then shifted to 34°C for 10 and 90 min. Cells were fixed in methanol for microscopy. (B) Percentage of cells with polarized Sec15-GFP. Small-budded cells from the above experiments were scored for the presence of Sec15-GFP at the bud tip (polarized) or lack of Sec15-GFP in the bud tip (mislocalized). (C) The initial targeting of Sec15-GFP to the bud tip is dependent on activated Sec4p. Wild-type, sec2-59, and sec4-8 cells expressing Sec15-GFP were arrested at G₀ and then released in fresh media for 90 min at 25°C (left) or 34°C (right). Cells were then fixed for microscopy. Bottom: Sec15-GFP; top: phase contrast images of the cells.

To further investigate the role of Sec4p in the initial targetingof Sec15p to the bud tip, we examined Sec15-GFP localizationin cells released from G₀. The yeast cells were isolated asa homogenous population arrested at G₀ (Ayscough et al., 1997).Releasing the cells from G₀ allowed us to examine the initialrecruitment of secretory machinery to the emerging bud for polarizedcell growth. We looked for polarization of Sec15-GFP in thetips of small buds or patches of Sec15-GFP at the cortexes representingincipient buds. As shown in Figure 1C, Sec15-GFP was localizedto small buds or incipient buds in wild-type cells releasedfrom G₀ at both 25°C and 34°C. In sec2-59 and sec4-8cells, Sec15-GFP formed patches in small buds and incipientbuds at 25°C. However, at 34°C many of the mutant cellsremain unbudded. Even in cells with small buds, Sec15-GFP wasnot concentrated to the bud. The lack of Sec15-GFP at buds inG₀ released mutant cells indicates that Sec4p and Sec2p functionsare required for the initial delivery of Sec15p to sites ofpolarized exocytosis.

The Localization of Sec15p in Cells Treated with Latrunculin
As shown above, the polarized localization of Sec15p requiresfunctional rab protein Sec4p. Because Sec4p associates withvesicle and is transported to the bud tip along actin cables(Walch-Solimena et al., 1997), we hypothesized that the abilityof Sec15p to polarize in yeast cells also requires polarizedactin organization. To test this hypothesis, we examined thelocalization of Sec15-GFP in cells treated with latrunculin-B(Lat-B), which disrupts the F-actin in yeast cells. Wild-typeyeast cells were grown to early log phase and then treated withLat-B to a final concentration of 200 or 400 µM. The yeastcells were cultured for an additional 30 min. A portion of thecells was collected for immunofluorescence staining of Sec4p.The remaining cells were fixed in methanol/acetone and examinedfor Sec15-GFP localization. As shown in Figure 2, Sec4p wascompletely mislocalized after Lat-B treatment. However, to oursurprise, Sec15-GFP was well polarized after treatment with200 or 400 µM Lat-B.

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Figure 2. The localization of Sec15p and Sec4p in cells treated with latrunculin. The localization of Sec4p, but not Sec15p, is disrupted by Lat-B treatment. Fluorescence images of Sec15-GFP (top panel) and immunofluorescence image of Sec4p (bottom panel) are shown for wild-type cells treated with DMSO (left), 200 µM Lat-B (middle), and 400 µM Lat-B (right) for 30 min.

A previous study showed that targeting of Sec3p to emergingbuds is independent of actin, as Sec3p remained a single "patch"at the plasma membrane even in cells released from G₀ underlatrunculin treatment (Finger et al., 1998). Here, we examinedthe localization of Sec15-GFP in yeast cells under the sameconditions (Figure 3). Wild-type yeast cells were isolated asa homogenous population arrested at G₀. An aliquot of cellswas released into fresh media in the presence of 200 µMLat-B or dimethyl sulfoxide (DMSO), as a control. As shown inFigure 3, actin cables were intact in cells treated with DMSO,and Sec15-GFP was localized to small buds in these cells. However,in the cells treated with Lat-B, most of the cells remainedunbudded. Actin cables were completely disrupted and Sec15-GFPcould not form any patch structures in the cells. After we recoveredthe cells in fresh media in the absence of Lat-B for 15 min,the cells began to form buds, and Sec15-GFP became polarizedin these cells. These results suggest that, unlike Sec3p, theinitial delivery of Sec15p to the site of polarized exocytosisrequires actin cables. It was shown previously that most ofendogenous Sec15p is distributed at the plasma membrane in yeastcells (Salminen and Novick, 1989; Bowser and Novick, 1991),whereas most of Sec4p is associated with secretory vesicles(Goud et al., 1988). The Sec15-GFP remaining at the bud tipsafter Lat-B treatment may reflect the plasma membrane pool ofSec15p, which is less sensitive to the disruption of F-actin.

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Figure 3. The initial targeting of Sec15p to the bud tip depends on actin cables. The initial targeting of Sec15p to the bud tips is disrupted by Lat-B. The Left and middle: the fluorescence images of Sec15-GFP in cells released from G₀ in the presence of DMSO and 200 µM Lat-B, respectively; right: the cells 15 min after recovery from Lat-B treatment with fresh medium. Bottom: the actin staining with phalloidin in these cells.

The Localization of Sec15p in Tropomyosin Mutant Cells
Lat-B treatment disrupts both actin cables and actin patchesin yeast cells. To better examine the role of actin cables inthe localization of Sec15p, we examined the localization ofSec15p in tpm1-2, tpm2 ${Delta}$ cells, which rapidly lose actin cablesupon shifting to restrictive temperature (Pruyne et al., 1998).The yeast cells were grown to early log phase and then shiftedto 34.5°C for periods of 10 and 60 min. Cells were fixedin methanol/acetone and examined for Sec15-GFP localization.In wild-type cells, Sec15-GFP was concentrated as a crescentat the tips of small buds at 25°C. It remained mostly polarizedafter shifting to 34.5°C for 10 and 60 min (Figure 4A).In contrast, Sec15-GFP was mislocalized from the bud tips inthe mutant cells after 10 min at 34.5°C. After 60 min, Sec15-GFPwas almost completely mislocalized. We also examined the localizationof Sec3-GFP under the same conditions (Figure 4B) and foundthat Sec3-GFP was only moderately depolarized after 10 min at34.5°C. After 60 min, Sec3-GFP remained mostly polarizedin the cells, consistent with the previous proposal that Sec3plocalization is independent of actin (Finger et al., 1998).

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Figure 4. The localization of Sec15p, Sec3p, and Sec4p to the bud tip in the tpm mutants. (A) Fluorescence image of Sec15-GFP in tpm2 ${Delta}$ (top) and tpm1-2, tpm2 ${Delta}$ (bottom) cells grown at 25°C, and the restrictive temperature 34.5°C for 10 and 60 min. (B) Fluorescence image of Sec3-GFP in tpm2 ${Delta}$ (top) and tpm1-2, tpm2 ${Delta}$ (bottom) cells grown at 25°C, and the restrictive temperature 34.5°C for 10 and 60 min. (C) Fluorescence image of Sec15-myc are shown for tpm2 ${Delta}$ (left) and tpm1-2, tpm2 ${Delta}$ (middle and right) cells. Cells were released from G₀ and grown for 2 h at 34.5°C (left and middle). A portion of tpm1-2, tpm2 ${Delta}$ cells was then shifted back to 25°C and recovered for 10 min (right).

To examine whether the initial targeting of Sec15p needs actincables, we examined Sec15p localization in tpm mutant cellsreleased from G₀ using immunofluorescence. As shown in Figure 4C,Sec15p was localized to small buds or incipient buds inwild-type cells released from G₀ at both 25°C and 34.5°C.In tpm1-2, tpm2 ${Delta}$ cells, Sec15 was polarized to the small budsand incipient buds at 25°C, but was not polarized at 34.5°C.Upon shifting the mutant cells back to 25°C for 10 min,Sec15p was repolarized to the small buds and incipient buds.These results suggest that actin cables are required for theinitial delivery of Sec15p to sites of polarized exocytosis.

The Rab GDI Mediates the Rapid Recycling of Sec4p from the Bud Tip
Although both Sec15p and Sec4p need polarized actin for theirdelivery to the daughter cell membrane, what accounts for theirdifferent responses to the latrunculin treatment (Figure 2)?One possibility is that the diffusion or recycling of Sec4pand Sec15p from the bud tip membrane is regulated differently.The recycling of the rab proteins from their target membranesis mediated by the GDI protein Sec19p (Garrett et al., 1994).We examined the localization of Sec4p and Sec15p in the sec19-1mutant. As shown in Figure 5, after shifting the sec19-1 mutantto the restrictive temperature (34°C) for 90 min, Sec4premained polarized at the buds. However, the polarization patternslightly changed. Instead of being concentrated at the bud tipas in the wild-type cells, Sec4p spread slightly toward theinner region. In some cases, the staining of Sec4p is even brighter.Sec19p is the GDI for all the rab proteins in yeast includingYpt1p that functions in the ER-to-Golgi stage of transport.Like the NSF protein Sec18p, Sec19p functions in every stageof traffic and mutations in Sec19p first block upstream ER-to-Golgitransport. It was shown previously that the localization ofSec4p relies on upstream traffic (Walch-Solimena et al., 1997).Mutations affecting early stages of traffic block the membraneflow to the post-Golgi stage, therefore affecting the transportof Sec4p by the secretory vesicles to its target membrane. AlthoughSec4p is diffused in all the early stage mutants, we show herethat it accumulated in the bud membrane in the sec19-1 mutant.Clearly, recycling of the GDP-bound form of Sec4p from the plasmamembrane depends on Sec19p.

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Figure 5. Effects of the rab GDI mutant (sec19-1) on the localization of Sec4p and Sec15p. Wild-type and sec19-1 cells were grown in SC-Ura media at 25°C and then shifted to 34°C for 90 min and fixed for microscopy. Sec15-GFP was mislocalized in the mutant cells (the bottom right panel). However, Sec4p accumulated near the bud tips in a "polarized" manner, although less concentrated comparing with those in the wild-type cells (the top right panel). Cells were then fixed for microscopy.

In contrast to Sec4p, Sec15p completely diffused in the sec19-1mutant at the restrictive temperature (Figure 5). The diffusionmay be attributed to the block of membrane traffic from earlystages or the failure of the recycling of GDP-Sec4p to GTP-Sec4p.We do not know what accounts for the diffusion or recyclingof Sec15p and the exocyst complex from the plasma membrane inwild-type cells.

The Localization of Sec15p and Sec4p Depends on Cdc42p
The Rho protein Cdc42p plays an essential role in the establishmentof cell polarity in yeast. Cdc42p controls the polarized organizationof actin cables, on which secretory vesicles are transportedto the bud (Dong et al., 2003). In addition, Cdc42p directlyinteracts with the exocyst protein Sec3p and deletion of theN-terminus Cdc42p binding domain (sec3 ${Delta}$ N) resulted in mislocalizationof Sec3p (Guo et al., 2001; Zhang et al., 2001). However, wealso noticed in our experiments that several exocyst proteins,including Sec15p, remain polarized in the sec3 ${Delta}$ N mutant (Guoet al., 2001; Guo laboratory, unpublished results). Here, weexamine the role of Cdc42p on the polarization of Sec15p andSec4p. We used Sec15-GFP and Sec4p immunofluorescence stainingto examine the localization of these two proteins in cdc42-201mutants. Because Cdc42 is activated in the cells by its GEFCdc24p, we also examined the localization of Sec15p and Sec4pin the cdc24-4 mutant. Yeast cells were grown to early log phaseand then shifted to the restrictive temperature of 37°Cfor 10 or 90 min before fixation. Sec15-GFP was polarized tothe bud tips of wild-type cells at both 25 and 37°C (Figure 6).In cdc42-201 and cdc24-4 mutant cells, Sec15-GFP was polarizedat the permissive temperature of 25°C but became diffusedafter 10 or 90 min at 37°C. Similarly, Sec4p was mislocalizedin cdc42-201 and cdc24-4 cells at 37°C. The depolarizationof these two proteins in both cdc42-201 and cdc24-4 suggeststhat active Cdc42p is necessary for the recruitment of Sec15pand Sec4p to the bud tip. Why Sec15p is depolarized in thesecells is unclear. However, it is unlikely that the depolarizationof Sec15p is a consequence of Sec3p mislocalization.

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Figure 6. Sec15p and Sec4p require functional Cdc42p for their polarized localization to the bud tip. Sec15-GFP (A) and Sec4p (B) cannot polarize to bud tips in cdc42-201 and cdc24-4 mutants. Sec15-GFP and Sec4p immunofluorescence images are paired with the phase contract images of the cells to the right.

The Localization of Sec15p and Sec4p in bem1 ${Delta}$ Cells
To further study the role of polarity determinants on the polarizationof Sec15p and Sec4p, we examined cells lacking Bem1p (bem1 ${Delta}$ ).Bem1p binds to a number of proteins such as Cdc42p, Cdc24p,Rsr1p/Bud1p, the PAK-like kinases Ste20p and Cla4p and thereforeis important for organizing the signaling molecules for theestablishment of cell polarity (Bender and Pringle, 1991, Chenevertet al., 1992; Leeuw et al., 1995; Park et al., 1997; Butty etal., 1998; Gulli et al., 2000; Bose et al., 2001; Butty et al.,2002; Irazoqui et al., 2003). Yeast cells with Bem1 deletionare viable but exhibit defects in actin organization and cellpolarity (Bender and Pringle, 1991, Chenevert et al., 1992).We used bem1 ${Delta}$ yeast cells to examine the role of this polarityprotein in Sec15p localization. The bem1 ${Delta}$ cells were grown toearly log phase at 25°C. These cells exhibited heterogeneousmorphological defects such as multibudded cells and extremelylarge cells, consistent with previous observations (Bender etal., 1991). In most of the cells, Sec15-GFP was mislocalized(unpublished data). In multi-budded cells, Sec15-GFP tendedto be preferentially concentrated in one or several of the buds(Figure 7A). In single budded cells, Sec15-GFP was localizedto the tip of the bud. (Figure 7A).

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Figure 7. Localization of Sec15-GFP and Sec4p in bem1 ${Delta}$ cells. (A) Localization of Sec15-GFP in bem1 ${Delta}$ cells in a heterogeneous population. (B) Bem1p is required for the initial targeting of Sec15-GFP to the bud tip. bem1 ${Delta}$ cells expressing Sec15-GFP were arrested at G₀. A homogeneous population of unbudded cells were released in fresh media at 25°C and fixed in methanol/acetone for microscopy. Sec15-GFP fluorescence images are paired with the phase contract images of the cells to the right.

It is possible that some bem1 ${Delta}$ cells may be sufficiently ableto initiate polarized growth while other cells are delayed orfail in this process, which leads to the observed heterogeneityin morphology. We reasoned that if we isolated a populationat the G₀ stage and examined the initial budding in the synchronizedcells, we might be able to see the effect of Bem1p more clearly.After isolating a G₀ population, we released the cells at 25°Cfor 2 h and then fixed them in methanol/acetone for microscopy.We found that, in the majority of the bem1 ${Delta}$ cells released fromG₀, Sec15-GFP was not polarized. Even in small budded cells,a large portion of Sec15p was not enriched in the buds (Figure 7B).On the basis of these results, we propose that Sec15p polarizationis facilitated by Bem1p during budding.

Localization of Cdc42p to the Bud Tip Requires Polarized Actin Cables and a Functional Secretory Pathway
Spatial regulation of exocytosis is mediated by the Rho familyof small GTPases and polarized cytoskeleton organization. Onthe other hand, membrane traffic may mediate the transport ofcell polarity regulators to the site of cell growth. Recentworks using GFP-tagged Cdc42p demonstrated that vesicle deliveryalong actin cables is important for symmetry breaking in yeast(Wedlich-Soldner et al., 2003, 2004). Here, we examined thelocalization of endogenous Cdc42p in yeast mutants defectivein polarized exocytosis. We first examined the localizationof Cdc42p in the sec mutants (sec4-8, sec5-24, and sec6-4).Yeast cells were grown to early log phase and then shifted to34°C for 10, 30, or 90 min before staining with affinity-purifiedanti-Cdc42p polyclonal antibodies. We especially focused onthe early stage budding cells (e.g., cells with tiny or smallbuds), where Cdc42p should be concentrated in the tip in wild-typecells. As shown in Figure 8, A and B, shifting the temperaturefor 10 min caused a loss of Cdc42p staining at the bud tip inthe wild-type as well as all the mutant cells. With a longerperiod of incubation at the restrictive temperature, the wild-typecells recovered Cdc42p polarization, appearing 40.3% polarizedafter 30 min at 34°C and near normal polarization (70%)after 90 min. In contrast, Cdc42p remained mislocalized in sec4-8,sec5-24, and sec6-4 cells after 30 and 90 min at the restrictivetemperature. The loss of Cdc42p localization 10 min after thetemperature shift probably resulted from the heat-shock responseas commonly observed in yeast cells (Delley and Hall, 1999).These localization studies suggest that Cdc42p, although itselfthe master regulator of cell polarity, requires the functionalexocytosis pathway for the maintenance of its polarization atthe bud tips. To further investigate the role of vesicle deliveryin Cdc42p localization, we also examined Cdc42p polarizationin the tpm1-2, tpm2 ${Delta}$ mutant (Figure 8, C and D), which rapidlyloses actin cables when shifted to 34.5°C (Pruyne et al.,1998). We found that Cdc42p was significantly depolarized after10 min (21% polarized) in the tpm1-2, tpm2 ${Delta}$ strain and graduallybecame even less polarized after 30 min (18% polarized) and90 min (7% polarized). We propose that Cdc42p requires a functionalsecretory pathway and polarized actin cables for the maintenanceof its localization at the buds.

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Figure 8. Polarization of endogenous Cdc42p requires functional secretory pathway and actin cable. (A) sec mutants disrupt Cdc42p polarization. Wild-type yeast (NY179), sec4-8, sec5-24, and sec6-4 (unpublished data) were grown in YPD to log phase and then shifted to 34°C for 10, 30, and 90 min. Cells were stained with affinity-purified ${alpha}$ -Cdc42p polyclonal antibodies. The Cdc42p immunofluorescence images are paired with the phase contract images of the cells to the right. Cells from the experiment were scored for polarization of Cdc42p to the bud tip (B). (C) Cdc42p is mislocalized in tpm1-2, tpm2 ${Delta}$ cells at the restrictive temperature of 34.5°C. Cells from C were scored for polarization of Cdc42p to the bud tip (D).

Bem1p Polarization Is Decreased in sec and tpm Mutants
Bem1p is important for the organization and assembly of a numberof signal proteins for bud emergence (Bender and Pringle, 1991,Chenevert et al., 1992; Gulli et al., 2000; Bose et al., 2001;Butty et al., 2002; Irazoqui et al., 2003). We expressed Bem1-GFPin the sec mutants to study the effect of exocytosis on thepolarization of Bem1p. The mutant yeast were grown to log phaseand then shifted to the restrictive temperature for 10 or 90min. We found that the number of cells with polarized Bem1-GFPdecreased over time (Figure 9A). Because Bem1-GFP fluorescencesignal was very weak in the tpm1-2, tpm2 ${Delta}$ mutant strain, we expressedBem1–12xmyc in this mutant for immunofluorescence staining.In a heterogeneous population shifted to 34.5°C for 10 min,Bem1p polarization decreased modestly to 60%. After 90 min thepercentage of polarized cells decreased further to 26%. Thisis different from that of Cdc42p, which decreased to 21% aftera 10-min shift and to <10% at a 90-min shift (Figure 8).So far, we were not able to perform double-labeling of the samecells to compare the localization of Bem1p and Cdc42p. However,the difference in the time course of depolarization for thetwo proteins is obvious.

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Figure 9. Bem1p polarization is affected in mutants defective in polarized exocytosis. (A) sec mutants affect Bem1p polarization. Wild-type, sec4-8, and sec2-59 strains expressing Bem1-GFP were grown in SC-Ura media to log phase and then shifted to the restrictive temperature for 10 min and 90 min. Cells were fixed in methanol/acetone for microscopy. (B) Cells from A were scored for polarization of Bem1-GFP to the bud tip. (C) Actin cables are necessary for Bem1p polarization. tpm2 ${Delta}$ and tpm1-2, tpm2 ${Delta}$ cells expressing Bem1–12xmyc were grown to log phase in YPD and then shifted to 34.5°C for 10 and 90 min. The cells were fixed and stained with ${alpha}$ -myc antibody to view the localization of Bem1p. Scoring of small budded cells with polarized Bem1p is shown in D. In addition, the localization of Bem1p in cells released from G0 was shown in the right panel of C.

To investigate the effect of actin cables on the initial deliveryof Bem1p to the bud tip, we examined Bem1-myc in tpm mutantsreleased from G₀ at the restrictive temperature. We found thatthe G₀ arrested cells were not able to polarize Bem1p when releasedat the restrictive temperature, although they could at the permissivetemperature. This result suggests that localization of Bem1pat the onset of the cell cycle needs the availability of functionalactin cable construction machinery.

The Exocyst Interacts with Bem1p
A number of yeast two-hybrid screenings revealed potential interactionbetween Sec15p and Bem1p (Drees et al., 2001; also see SGD formore references). In the screening performed by the yeast polarityconsortium, positive interaction was found between Sec15p andCdc24p in addition to Bem1p (Drees et al., 2001). Cdc24p wasshown to bind the PB1 domain of Bem1p (Gulli et al., 2000; Buttyet al., 2002; Yoshinaga et al., 2003). The two-hybrid resultmay reflect an indirect interaction between Sec15p with Cdc24pthrough Bem1p. To test whether Sec15p interacts with Bem1p invivo, GST-Bem1p was expressed in a yeast strain with its endogenousSec15 (the chromosomal copy) tagged by the myc epitope (Sec15p-myc).Pull-down experiments were performed using glutathione-Sepharose.As shown in Figure 10, Sec15p coprecipitates with GST-Bem1p.In addition, Sec8p, another exocyst component, also coprecipitates,suggesting that the exocyst complex interacts with Bem1p inthe cell. As a control, GST does not bind to Sec15p or Sec8p.Using this assay, we also found that Cdc24p coprecipitates withBem1p, consistent with previous observations. Although detailedprotein-protein interactions of the exocyst with Bem1p and Cdc24pare unclear, our result suggests that the exocyst interactswith Bem1p in vivo.

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Figure 10. Bem1p interacts with Sec15p and Sec8p in vivo. GST-Bem1p or GST (as control) was coexpressed with myc-tagged Sec15p, Sec8p, or GFP-tagged Cdc24p in yeast cells. The same amounts of lysates from these strains were used for coprecipitation with glutathione-Sepharose 4B to test the interaction between Bem1p and the exocyst proteins. The precipitates were separated by SDS-PAGE and subjected to Western blot analyses using anti-GST antibody to detect GST and GST-Bem1p (left panel), anti-myc antibody to detect Sec15-myc and Sec8-myc, and anti-GFP antibody to detect Cdc24-GFP (Bound, bottom right panel).

DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

Localization of a protein to the bud tip represents a balancebetween targeting of the protein to this region, and diffusionor recycling of the protein from this site. The exocyst proteinSec15p is a direct downstream effector of Sec4p (Guo et al.,1999b). We show here that the localization of Sec15p to thebud tip requires active Sec4p, suggesting that Sec4p controlsthe delivery and/or assembly of the exocyst complex at the bud.But in contrast to Sec4p, treatment of cells with latrunculindoes not affect Sec15p localization. The initial targeting ofSec15p needs actin cables as Sec15p could not be found in theemerging buds in the tpm mutant cells released from G₀. However,once Sec15p reaches its destination, its association with theplasma membrane seems to be quite stable. This hypothesis isconsistent with the previous biochemical fractionation datathat the majority of the endogenous Sec15p is associated withthe plasma membrane (Bowser and Novick, 1991) even though Sec15pclearly has the ability to associate with the vesicles (Salminenand Novick, 1989; Guo et al., 1999b). The rab protein Sec4pis also targeted to the bud along actin cables (Walch-Solimenaet al., 1997; Pruyne et al., 1998). However, unlike Sec15p,Sec4p is rapidly depolarized in the presence of latrunculin(Figure 2; also see Ayscough et al., 1997) or in the tpm mutantshifted to the restrictive temperature (Pruyne et al., 1998).GTP-loaded Sec4p is transported via post-Golgi vesicles to theplasma membrane. Once reaching the bud tip membrane, its GAPs,Msb3p and Msb4p, promote GTP hydrolysis and Sec4p becomes GDP-bound(Gao et al., 2003) at the bud. The GDP-bound form of Sec4p isthen extracted from the lipids by Sec19p, the GDI for the rabGTPases, for subsequent recycling (Garrett et al., 1994). Sec19pnot only regulates Sec4p, its GDI function is toward all therab proteins at different stages of membrane traffic. Therefore,in sec19 mutants, early stage trafficking defects were alsodetected (Novick et al., 1980). It has been shown that polarizedSec4p localization needs functional upstream traffic (Walch-Solimenaet al., 1997). However, in the sec19 mutant, Sec4p accumulatesin the bud (Figure 5). This result suggests that the recyclingof Sec4-GDP was blocked in the GDI mutant; therefore the remainingSec4p was accumulated in the bud in a seemingly "polarized"manner. We have also treated the sec19-1 mutant cells by latrunculinand examined the localization of Sec4p in these cells. We expectthat Sec4p will not be accumulated in the buds in sec19-1 cellsas both the targeting and recycling of Sec4p are blocked. Weindeed observed the loss of Sec4p in the bud (unpublished data).However, we also found that DMSO (used to dissolve latrunculin,as a control) treatment alone led to Sec4p delocalization in $~$ 40% of the sec19-1 cells. One possibility is that DMSO, as anorganic solvent, may modify the lipids in the plasma membrane,therefore complicating our interpretation of the GDI functionat the plasma membrane.

The recycling of Sec4p in the presence of functional GDI isa fast process compared with that of Sec15p, as disruption ofthe actin cytoskeleton by latrunculin leads to rapid depolarizationof Sec4p but not Sec15p. Sec15p, though controlled by Sec4p,is mislocalized in the GDI mutant. This mislocalization probablyresulted from disruption of upstream trafficking in the sec19mutant. The mechanisms for the recycling or diffusion of Sec15pand other exocyst proteins are unknown. Future experiments areneeded to address this question.

We have also compared the localization of Sec15p with anotherexocyst protein, Sec3p, in the cells. The relationship betweenSec3p and actin was rigorously tested previously (Finger etal., 1998). Like Sec15p, the maintenance of Sec3p at the budtip is not sensitive to latrunculin treatment. However, thetargeting of Sec3p was also shown to be independent of actinas Sec3-GFP can be targeted as a patch-like structure even inG₀ released cells in the presence of latrunculin (Finger etal., 1998). Also in the tpm mutant cells, Sec3p is much morestable than Sec15p at the bud tip, remaining mostly polarizedafter a 90-min shift to the restrictive temperature (Figure 4).The time course of Sec15p localization closely resemblesthat of Sec8p in the tpm mutant previously reported (Pruyneet al., 1998; Guo laboratory, unpublished results). These resultsrevealed that different mechanisms direct the targeting of Sec3pversus other members of the exocyst complex. We previously foundthat Cdc42p and Rho1p control the localization of Sec3p throughtheir interaction with the N-terminus of Sec3p (Guo et al.,2001; Zhang et al., 2001). Rho1p and Cdc42p compete with eachother in their binding to this region of Sec3p (Zhang et al.,2001). This interaction is necessary for the polarized localizationof Sec3p, as deletion of the N-terminus of Sec3p (Sec3 ${Delta}$ N) leadsto mislocalization of Sec3p without affecting the assembly ofthe exocyst complex (Guo et al., 2001). Interestingly, in thesec3 ${Delta}$ N mutant strain, Sec15p is still polarized (Guo laboratory,unpublished results). Therefore, there must be parallel pathwaysthat target different exocyst components to sites of activesecretion. Here we demonstrate that Cdc42p controls Sec15p localizationin the cells (Figure 6) similar to Sec3p. Although Cdc42p controlsSec3p localization through its direct binding with Sec3p N-terminus,its role for Sec15p and other exocyst components must be mediatedthrough a Sec3p-independent pathway. Future works are neededto further compare these proteins in the same cells using time-lapsemicroscopy so that their kinetics differences can be betterstudied. These results revealed the diversity of exocyst targetingin yeast cells. As the exocyst functions in a step proceedingSNARE-mediated membrane fusion, the eight proteins are targetsfor cellular regulators (Lipschutz and Mostov, 2002; Novickand Guo, 2002; Hsu et al., 2004). The assembly of the exocystmay integrate various sources of cellular information to ensurethat exocytosis occurs at the right time and place.

Although our studies demonstrate that the post-Golgi secretorymachinery is under the control of the actin cytoskeleton andpolarity regulators, we also examined the localization of thepolarity determinants in cells defective in exocytosis. We hypothesizethat membrane traffic may be important for the delivery of polarityregulators to specific domains of the plasma membrane. We firstexamined Cdc42p, the "master" regulator for the establishmentof polarity in yeast. Using affinity-purified antibodies, wefound that the localization of endogenous Cdc42p at sites ofpolarized cell growth relies on a functional secretory pathway,as the sec mutant cells lose Cdc42p staining at the bud tipover time. Cdc42p localization also needs actin cables, whichare essential for polarized transport of secretory vesicles.Disruption of actin cables in the tpm mutant results in lossof polarized localization of Cdc42p, consistent with the observationby Pruyne et al. (2004). Recently, Wedlich-Soldner et al. (2003,2004) demonstrated that polarized localization of GFP-taggedCdc42p required targeted secretion directed by the actin cytoskeleton.It was proposed that the F-actin–dependent transport ofCdc42p to the plasma membrane, which in turn is controlled byCdc42p, provides a positive feedback loop that amplifies initialsmall signals for symmetry breaking in the early stages of yeastbudding. Our study demonstrates that Cdc42p loses its localizationin the established buds in exocytosis mutants. Our results suggestthat a functional secretory pathway and actin cables are notonly needed for bud emergence, but are also important for maintainingthe localization of Cdc42p in the growing bud. Biochemical experiments(Wedlich-Soldner et al., 2003, 2004) suggest that Cdc42p associateswith secretory vesicles. It is possible that continued replenishmentof Cdc42p to the bud to counter the endocytosis of bud membraneis important for the maintenance of Cdc42p at sites of cellpolarization.

The function of Cdc42p is carried out in conjunction with Bem1p,which interacts with Cdc42p, its GEF Cdc24p, and other signalingmolecules involved in cell polarity establishment. Here we foundthat Bem1p also loses its polarized localization in the secand tpm mutants, suggesting that the maintenance of Bem1p requirespolarized transport. However, the time course of Bem1p depolarizationis slower than that of Cdc42p. Especially, the slow depolarizationof Bem1p in the tpm mutant, which is known to rapidly lose cablesafter 1 min (Pruyne et al., 1998), suggests that loss of actincables affects Bem1p polarization indirectly over time. It ispossible that the diffusion or recycling of Bem1p from the budtakes a time course different from Cdc42p. A recent findingsuggests that the self-assembly of Bem1p leads to scaffold-mediatedsymmetry breaking in yeast (Irazoqui et al., 2003). It is possiblethat the mislocalization of Bem1p observed in our study resultedindirectly from Cdc42p mislocalization in the mutants. BesidesBem1p, it was reported that proteins regulating actin polymerization,the motor protein Myo2p, and actin itself are disrupted in secretorymutants (Jin and Amberg, 2000; Gao et al., 2003; Aronov andGerst, 2004; Pruyne et al., 2004). Overall these studies presenta cyclical regulatory mechanism that may be important for theestablishment and maintenance of polarized cell growth. In thisregard, it is interesting to note that several yeast two-hybridscreenings from different sources revealed potential interactionsbetween Sec15p and Bem1p (Drees et al., 2001; also see SGD formore references). Here, we demonstrated that Sec15p indeed interactswith Bem1p in yeast cells. We have previously shown that Cdc42pdirectly interacts with Sec3p (Zhang et al., 2001). Stringentcytological experiments suggest that Sec3p, unlike the otherexocyst components, is not dependent on actin for its polarizedlocalization (Finger et al., 1998). Sec3p may associate withthe plasma membrane and then assemble with other exocyst proteins,including Sec15p, that arrive at the bud tip via secretory vesiclesalong the actin cables (Finger and Novick, 1998). The interactionof Sec15p with Bem1p and its assembly into the exocyst complexbring Cdc42p, its exchange factor Cdc24p, and the Cdc42p effectorSec3p into close proximity at the bud tip. These molecular interactionsmay represent a positive feedback loop coupling vesicle deliveryand cell polarization. However, to test this hypothesis, themolecular details of the interactions clearly need to be elucidatedfirst.

If secretion is important for the polarized localization ofcell polarity regulators, why were cell morphology defects notobserved in sec mutants? Most of the sec mutants previouslyisolated were "tight" alleles. On shifting to the restrictivetemperature, bud emergence stopped quickly, as indicated bythe nearly constant number of cells and buds (Novick et al.,1980). In a heterogeneous population, cells were found to arrestat all stages of cell cycle, and no significant increase incell size was noted (Novick et al., 1980; Guo laboratory, unpublishedobservation). These characteristics of these sec alleles areresults of the screening strategy: only "dense" cells in whichnet cell surface growth stopped while cell mass increased, wereselected (Novick et al., 1980). Identification of new allelesof exocyst mutants may help reveal defects in both secretionand morphogenesis.

This cyclical regulatory mechanism between secretion and cellpolarity has been observed in mammals. One recent example waspresented by O'Brien et al. (2001). The authors demonstratedan autocrine loop, in which epithelial cells create their ownextracellular polarity cue through exocytosis during cystogenesis.The secretion and assembly of extracellular laminin acts backon the cells to direct membrane traffic. Blocking the activityof the small GTPase Rac1 disrupts the loop, which leads to aninversion of the apical pole. Future studies using a varietyof model systems will help us better understand the molecularbasis and biological consequences underlying this cyclical regulatorymechanism.

ACKNOWLEDGMENTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
ACKNOWLEDGMENTS
REFERENCES

We are grateful to Drs. Erfei Bi, Tony Bretscher, and AllanBender for valuable reagents. Especially, we are grateful toDr. Keith Kozminski for the affinity-purified anti-Cdc42p antibodies.We thank Dr. Erfei Bi for many helpful discussions and Dr. PeterNovick for the communications of data before publication. Thiswork is supported by grants from the National Institutes ofHealth, American Cancer Society, and Pew Scholar Program inBiomedical Sciences to W.G.

Footnotes

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E04-10-0896)on January 12, 2005.

The authors declare that they have no competing financial interests.

^* These authors contributed equally to this work.

Address correspondence to: Wei Guo (guowei{at}sas.upenn.edu).

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