SNARE Membrane Trafficking Dynamics In Vivo

doi:10.1083/jcb.144.5.869

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© The Rockefeller University Press, 0021-9525/1999//869 $5.00
The Journal of Cell Biology, Volume 144, Number 5, , 1999 869-881

Regular Articles

SNARE Membrane Trafficking Dynamics In Vivo

Daniel S. Chao^*, Jesse C. Hay^*, Shawn Winnick^*, Rytis Prekeris^*, Judith Klumperman, and Richard H. Scheller^*

^* Howard Hughes Medical Institute, Department of Molecular and Cellular Physiology, Stanford University School of Medicine, Stanford, California 94305-5428; and Medical School, Institute for Biomembranes, University of Utrecht, 3584CX Utrecht, The Netherlands

The ER/Golgi soluble NSF attachment protein receptor (SNARE)membrin, rsec22b, and rbet1 are enriched in $~$ 1-µm cytoplasmicstructures that lie very close to the ER. These appear to beER exit sites since secretory cargo concentrates in and exitsfrom these structures. rsec22b and rbet1 fused to fluorescent proteins are enriched at $~$ 1-µm ER exit sites that remainedmore or less stationary, but periodically emitted streaks offluorescence that traveled generally in the direction of theGolgi complex. These exit sites were reused and subsequent tubulesor streams of vesicles followed similar trajectories. Fluorescentmembrin- enriched $~$ 1-µm peripheral structures were moremobile and appeared to translocate through the cytoplasm backand forth, between the periphery and the Golgi area. Thesemobile structures could serve to collect secretory cargo byfusing with ER-derived vesicles and ferrying the cargo to theGolgi. The post-Golgi SNAREs, syntaxin 6 and syntaxin 13, whenfused to fluorescent proteins each displayed characteristicpatterns of movement. However, syntaxin 13 was the only SNAREwhose life cycle appeared to involve interactions with the plasmamembrane. These studies reveal the in vivo spatiotemporal dynamicsof SNARE proteins and provide new insight into their roles inmembrane trafficking.

Key Words: vesicle trafficking • fluorescent proteins • SNAREs • membrane proteins • endoplasmic reticulum

Abbreviations used in this paper: B,C,G,Y FP, blue, cyan, green, yellow fluorescent protein; IC, intermediate compartment; NRK, normal rat kidney; NSF, N-ethylmaleimide-sensitive factor; SNAP-25, synaptosome-associated protein of 25 kD; SNAP, soluble NSF attachment protein; SNARE, soluble NSF attachment protein receptor; VAMP, vesicle-associated membrane protein; ts-G-GFP, temperature sensitive vesicular stomatitis virus-associated membrane protein; VTC, vesicular tubular cluster.

DISTINCT membrane compartments of the secretory pathway aremaintained despite the continuous anterograde and retrogradeflow of proteins and lipids throughout the cell. This is accomplishedby an intricate series of membrane trafficking decisions includingthe concentration and packaging of cargo and the organized fusion of specific membranes. Understanding the molecular mechanismsunderlying membrane trafficking decisions will greatly furtherour appreciation of cellular regulatory mechanisms.

One particularly interesting aspect of membrane traffickingis the specificity and mechanism of the membrane fusion process.Studies in yeast (Alto et al., 1993; Brennwald et al., 1994)and the mammalian nerve terminal have defined a set of proteinscritical for membrane fusion (Bennett and Scheller, 1993).Vesicle-associated membrane protein (VAMP),¹ syntaxin, and synaptosome-associatedprotein of 25 kD (SNAP-25), collectively referred to as solubleNSF attachment protein receptors (SNAREs) (Söllner et al., 1993a),are the prototypes of a class of integral membrane (VAMP andsyntaxin) or lipid modified (SNAP-25) proteins of the vesicleand plasma membrane. The binding of vesicle- and target-SNAREs(v- and t-SNAREs, respectively) from opposite membranes (Nichols et al., 1997) is critical in the fusion process because formation of this complex brings the bilayer in close proximity and possibly even drives the fusion process itself (Hanson et al., 1997; Lin and Scheller, 1997).

The v- and t-SNARE complex referred to as the core complexdissociates in a two-step process. First, two soluble factors, ${alpha}$ SNAP and N-ethylmaleimide-sensitive factor, bind the core complex,resulting in a 20S particle. Upon ATP hydrolysis by N-ethylmaleimide-sensitivefactor, the v-SNARE dissociates from the complex (Söllner et al., 1993b),allowing the SNAREs to participate in another round of membranefusion (Mayer et al., 1996). Recent studies have uncovered alarge number of VAMP and syntaxin homologues and these proteinsare specifically localized to many different compartments withinthe cell (Wang et al., 1997; Advani et al., 1998). The possibility that the specific pairing of v- and t-SNAREs may be a criticaldeterminant of the specificity of membrane fusion has beenwidely discussed (Rothman and Warren, 1994) but remains a largelyuntested hypothesis.

Although many other proteins, thought to function upstream ofcore complex formation, are critical in the vesicle traffickingprocess their specific roles are less well understood. Forexample, members of the Rab family of GTPases are specificallylocalized on many different membranes and have been demonstratedto be critical in the trafficking process (Pfeffer, 1996; Novick and Zerial, 1997).In addition, the sec1 family of syntaxin binding proteins isrequired for membrane fusion. While the sec1 family appearsto be smaller than the syntaxin family, clear specificity inthe associations between members of these protein familieshas been demonstrated (Pevsner et al., 1994). Also synaptotagminand CAPS have been proposed to represent sensors for Ca²⁺ thatregulates the final step of exocytosis (Südhof, 1995;Loyet et al., 1998). Further studies of these molecules promisesto illuminate the biochemical mechanisms of membrane traffickingand exocytosis.

While genetic, biochemical, and immunohistochemical techniquesprovide important mechanistic insight into membrane trafficking,they provide little information on the dynamics of organellesin living cells. Several studies have investigated the dynamicsof membrane trafficking in living cells using fluorescent dyes.Some of these dyes specifically stain particular domains ofthe secretory pathway. For example, NBD-ceramide, a vital stainof the TGN, has been used to reveal dynamic tubulovesicularprocesses that emerge from the TGN extending along microtubules where they contact adjacent Golgi elements (Cooper et al., 1990).More recently, green fluorescent protein (GFP) has been fusedto proteins that travel through the secretory pathway in orderto observe their trafficking pathways. A particularly usefulmarker for following trafficking pathways has been the temperature-sensitivemutant viral glycoprotein VSVGtsO45 (Bergmann, 1989) fusedto GFP (ts-G-GFP). At the nonpermissive temperature this constructis misfolded and retained in the ER, whereas at the permissivetemperature the ts-G-GFP is correctly routed through the Golgicomplex to the plasma membrane (Presley et al., 1998). Imagingof ts-G-GFP uncovered an extensive network of tubulovesicularmembranes interposed between the ER and the Golgi complex.These studies also revealed large $~$ 1-µm structures calledvesicular tubular clusters (VTCs) that move from the periphery to the Golgi region (Balch et al., 1994; Presley et al., 1997; Sciaky et al., 1997; Cole et al., 1998). Similar techniques have also been used to demonstrate sequential roles of COPIIand COPI coats in ER to Golgi trafficking (Scales et al., 1997).

In this study we use a variety of antibodies and GFP fusionproteins to study the dynamics of SNARE proteins and the traffickingpathways they mediate within the secretory pathway (see Fig.1). We had generated previously a useful set of mAbs and pAbsto the cytoplasmic domains of several SNARE proteins (Hay et al., 1998).As additional markers to identify the ER, we used antibodies that recognized calnexin and Bip. We tracked the flow of cargousing ts-G-GFP. The dynamics of individual SNARE proteins wasinvestigated in vivo using either blue, cyan, green, or yellowfluorescent proteins (BFP, CFP, GFP, YFP, respectively) fusedto the lumenal or cytoplasmic domains of the SNAREs. We revealrsec22b- and rbet1-enriched ER exit sites from which vesiclesand/ or tubules emanate. Movement of these vesicles/tubulesis generally directed towards the Golgi complex. Other pre-GolgiSNAREs displayed different behaviors. Membrin is concentratedin dynamic 1-µm structures, whereas GOS-28 appears restrictedto the Golgi and remains relatively static. Post-Golgi SNAREsshow distinct and extremely dynamic trafficking pathways. Byusing cyan and yellow fluorescent fusion proteins transfectedinto the same cell the intersection of the distinct traffickingpathways is observed. The unique dynamics of each SNARE-FP–labeled organelle likely requires specific coupling to motors and cytoskeletal tracks. Consequently, this process plays an importantrole in determining the specificity of protein traffickingand membrane fusion.

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Figure 1 Schematic of reagents used in this study. mAbs and pAbs against the cytoplasmic domains of several SNARE proteins were characterized previously. Antibodies against Bip and calnexin were used to identify the ER. The temperature-sensitive form of VSV-G coupled to fluorescent proteins serves as a secretory pathway cargo visible in living cells. B, C, G, and YFP were fused to a variety of SNARE proteins. Coupling to the NH₂-terminal of the SNARE results in a fluorescent protein exposed to the cytoplasm, whereas fusion to the COOH-terminal end places the fluorescent protein within the lumen.

	Materials and Methods

Top Abstract Materials and Methods Results Discussion References

Immunofluorescence Microscopy of Fixed Normal Rat Kidney (NRK) Cells
NRK cells were maintained in DME containing 5 g glucose perliter, 10% FCS, and antibiotics in a humidified 5% CO₂ incubator.For transfection with ts-G-GFP (slight modification of Scales et al., 1997)all of the following occurred: one barely confluent 10-cm dishof NRK cells, $~$ 10⁷ cells, was removed from the plate with trypsin-EDTA,washed once with PBS, resuspended in 0.6 ml of PBS, and incubatedfor 10 min on ice with 10 µg of plasmid DNA in a 0.4-cmgap electroporation cell (Bio-Rad Laboratories). The cells wereelectroporated using 960 µF and 0.25 kV in an electroporator(Bio-Rad Laboratories) with capacitance extender, and plated on 2.2-cm² glass coverslips. After 5 h at 37°C, sodiumbutyrate was added to 5 mM and the cells were shifted to 40°Cfor 12 h. For microscopy, coverslips (from control nontransfectedcells at 37°C or transfected cells at 40°C) were eitherdropped directly into a well containing 4% paraformaldehyde,0.1 M sodium phosphate, pH 7.0, or dropped into wells of mediumpreequilibrated at 32°C, and incubated for various lengthsof time before fixation. After 30 min of fixation, coverslipswere moved to wells containing 0.1 M glycine in PBS for >10min, and equilibrated in permeabilization buffer (PBS containing0.4% saponin, 1% BSA, and 2% normal goat serum). Staining wascarried out at room temperature for 1 h in a permeabilizationsolution containing combinations of a calnexin polyclonal antiserum(Hammond and Helenius, 1994), a commercial rabbit polyclonalantibody to Bip (Stressgen), the affinity-purified rabbit anti–rat membrin 2-125 (Hay et al., 1998) or rbet1 mAb 16G6 (Hay et al., 1998). Coverslips were washed three times for 15 min each in permeabilization buffer and incubated for 30 min with anti–rabbit or anti–mousesecondary antibodies conjugated to FITC or Texas red. For stainingwith one of these antisera relative to GFP-G protein, Texasred secondary was used for staining so that it could be detectedrelative to the inherent green fluorescence of the GFP-G protein.After washing with permeabilization solution as above, coverslipswere mounted in mounting medium (Vectashield; Vector Laboratories)and viewed using a fluorescence microscope (Olympus IX70; OlympusOptical Co.) with a 100x oil immersion lens, an image acquisitionsystem (DeltaVision; Applied Precision), and a computer (modelO2; Silicon Graphics). Images were captured to disk using filtersets appropriate for FITC (for FITC or GFP fluorescence) or Texas red (for Texas red fluorescence). Images were cropped,adjusted, and arranged using Adobe Photoshop and printed ona photodigital printer (Fujix Pictography; Fuji Photo FilmCo.). Colocalization was quantitated blindly by placing punctainto three categories: SNARE alone, ts-G-VSV alone, or SNAREand ts-G-VSV. From each time point at least 50 puncta werecategorized.

Immunogold Labeling of Ultrathin Cryosections
HepG2 cells were fixed in a mixture of 2% formaldehyde and 0.2%glutaraldehyde in 0.1 M phosphate buffer, pH 7.4, and preparedfor cryosectioning and double-immunogold labeling accordingto the protein A gold method as described (Slot et al., 1991;Liou et al., 1996; Hay et al., 1998).

Construction of Fluorescent Protein Fusions
Coding regions of SNAREs were amplified using PCR and clonedin frame into pEGFP-N3 or pEGFP-C1 (CLONTECH Laboratories,Inc.). EYFP, ECFP, and EBFP (CLONTECH Laboratories, Inc.) coding regions were amplified using PCR and cloned into pEGFP-N3 and pEGFP-C1 lacking GFP to produce pEYFP-N3, pEYFP-C1, pECFP-N3, pECFP-C1, pEBFP-N3, and pEBFP-C1 mammalian expression vectors (collectively called pEFP). Coding regions from each SNAREwere cut from pEGFP-N3-SNARE and pEGFP-C1-SNARE and ligatedinto various pEFP vectors. All PCR-amplified inserts were sequencedto ensure no mutations were introduced. VSV-G-ts045 codingregion was cut from VSV-G-ts-045-GFP (Scales et al., 1997)and ligated into various pEFP-N3 constructs.

Time-Lapse Imaging
NRK cells were electroporated with 7 µg plasmid DNA forsingle-transfected or 5 µg of each plasmid for double-transfectedcells and plated onto glass coverslips one day before imagingas previously described. Coverslips with transfected cells weretransferred to an imaging chamber (Warner Instruments) containingDME without phenol red supplemented with 25 mM Hepes, pH 7.4,10% FCS, 1x penicillin/streptomycin. Cells were visualizedwith an inverted microscope (Olympus IX70; Olympus AmericaInc.) and a 60x or 100x oil immersion objective. The entiremicroscope was enclosed in a plastic chamber and prewarmed toeither 32°C for VSV-FP movies, or 37°C for movies notinvolving VSV. Images were acquired using a CCD camera andDeltaVision software every 1.5–4 s with 0.3–1.0-sexposure times for up to 100 exposures for single- and 200 exposures for double-transfected cells. An FITC filter set wasused for GFP movies and a custom made CFP/YFP excitation/emissionfilter set and polychroic was used for two-color CFP and YFPmovies (Chroma Technologies Corp.). Resulting movies were analyzedon a computer (octane; Silicon Graphics) and DeltaVision imageanalysis software.

Results

Top
Abstract
Materials and Methods
Results
Discussion
References

Punctuate Structures Containing rbet1 and Membrin Are ER Exit Sites
Previous immunofluorescence studies (Hay et al., 1998) localizedSNAREs (syntaxin 5, membrin, rsec22b, and rbet1) to the ER,Golgi, and numerous punctate structures throughout the cytoplasm.Immuno-EM established the identity of the punctate structuresas VTCs of the peripheral and Golgi-adjacent ER–Golgiintermediate compartment (IC). To further characterize theseelements and investigate their role as intermediates in secretorycargo transport, we employed double-label immunofluorescence microscopy experiments using ts-G-GFP and antibodies thatspecifically recognize SNAREs (Fig. 1).

First, we examined the relative distributions of endogenousrbet1 and membrin in fixed NRK cells. As shown in Fig. 2 (top),both proteins heavily labeled the juxtanuclear Golgi area aswell as small punctate structures throughout the cytoplasm.These steady-state, 37°C structures are similar to thosethat were observed to contain rbet1, rsec22b, and membrin afterincubations at 15°C. The difference is that at 15°C,these peripheral structures become markedly more intense relativeto juxtanuclear staining and their size increases (not shown).As documented previously (Hay et al., 1998), rbet1 and rsec22bare present at higher levels in the ER than membrin. Althoughmany bright cytoplasmic structures containing rbet1 also contained membrin (Fig. 2, top, arrows), VTCs were also visible that contained one but not the other of the two, suggesting somedifferentiation in their functions (see arrowheads).

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Figure 2 Peripheral structures containing both rbet1 and membrin are closely associated with, yet distinct from, ER tubules in fixed NRK cells. (Top row) Wild-type NRK cells grown at 37°C were fixed and stained for rbet1 (left) and membrin (middle) as described in Materials and Methods. Arrows represent peripheral structures positive for both proteins. Arrowheads represent peripheral structures positive for one, but not the other protein. (Middle row) Wild-type NRK cells grown at 37°C were fixed and stained for calnexin (left) and rbet1 (middle). (Bottom row) Wild-type NRK cells grown at 37°C were fixed and stained for Bip (left) and rbet1 (middle). Arrows in the middle and bottom rows point out peripheral rbet1- or membrin-positive structures very near, but distinct from, ER tubules. For Figs. 2, 4, and 5, the third column represents the merging of the first and second images. Bars, 10 µm (relative to objects in the first and second columns) and 4.3 µm (relative to insets). Insets show a higher magnification image from a similar cell.

Next we investigated whether the VTCs containing rbet1 andmembrin were closely associated with ER elements by costainingwith antibodies against resident ER proteins. We focused onperipheral VTCs because the density of membranes in the centralGolgi area of the cell is too high to observe distinct VTCs.As shown in Fig. 2 (middle) many rbet1-containing elementswere closely associated with ER tubules marked with calnexin,an integral membrane ER chaperone. Some of the rbet1 foci actuallyexclude or were de-enriched for calnexin (see arrows). Despitetheir apparent distinctness, the exclusive rbet1 elements andER tubules appeared conspicuously associated, since the rbet1spots were usually arranged in very close proximity to ER tubules.This is consistent with at least a portion of the rbet1-containingspots representing structures situated downstream of the sortingof secretory cargo away from ER resident proteins. These VTCs may originate adjacent to the ER by local fusion of ER-derivedvesicles. We occasionally observed rbet1 spots that were notimmediately adjacent to ER tubules (see Fig. 4, middle), perhapsrepresenting more mature VTCs en route to the Golgi area. AnotherER marker, Bip, displayed a similar overall staining patternas calnexin; it also shared only limited overlap with rbet1in the peripheral VTCs (Fig. 2, bottom, arrows).

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Figure 4 Secretory cargo retained in the ER has access to a subset of peripheral structures containing rbet1 and membrin. (Top row) ts-G-GFP– transfected NRK cells grown at 40°C were fixed and the subcellular distribution of ts-G-GFP protein (left) was compared to the calnexin staining pattern (middle). (Middle row) ts-G-GFP–transfected NRK cells grown at 40°C were fixed and the subcellular distribution of ts-G-GFP (left) was compared to the rbet1 staining pattern (middle). (Bottom row) ts-G-GFP–transfected NRK cells grown at 40°C were fixed and the subcellular distribution of ts-G-GFP (left) was compared to the membrin staining pattern (middle). Right column represents an overlay of the previous two images in the row. Arrows point out peripheral rbet1- or membrin-containing structures that did not contain a significant amount of ts-G-GFP protein, although they were adjacent to ER tubules. The arrowheads demonstrate that some of the exclusive structures were not immediately adjacent to ER tubules, perhaps representing mobile VTCs en route to the Golgi complex. Bars: (frames) 10 µm; (inset) 4.3 µm.

The organization of these SNARE-enriched foci was investigatedat higher resolution using immuno-EM and examples are shownof the labeling observed with rsec22b and COPII antibodies(Fig. 3). COPII coat proteins are present on anterograde-directedtransport vesicles that bud from the ER. Several conclusionsare drawn from these micrographs. First, no difference is observedin the organization of these sites when they are labeled withantibodies that recognize rbet1, rsec22b, or membrin, consistentwith the colocalization of the spotty immunoreactivity at thelight level. Second, sites close to the nucleus and those locatedclose to the plasma membrane have the same general organization.Third, the structures are comprised of an intricate networkof vesicles and/or tubules, and many are immunoreactive forboth the SNAREs and COPII. It is not possible to discern whetherlong tubules emanate from the ER traveling in and out of theplane of section, or, alternatively, if the observed elementsrepresent a myriad of individual vesicles. Finally, as is notedat the light level, these structures are adjacent to clearlyrecognizable ER cisternae.

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Figure 3 COPII and rsec22b immunogold labeling of peripheral ER exit sites. Ultrathin cryosections of HepG2 cells double-immunogold–labeled for COPII (10 nm gold) and rsec22b (15 nm gold). (A) ER exit sites (arrowheads) with similar morphology are present near the nucleus, N, and close to the plasma membrane, P. (B) A higher magnification of a peripheral ER exit site showing the characteristic tubulovesicular morphology. M, mitochondrion. Bars, 200 nm.

To help clarify the relationship of the SNARE-containing structuresto secretory cargo, we used a GFP-tagged version of VSV-G-ts045(ts-G-GFP) as a model ER-to-Golgi cargo protein (Fig. 1). Thetemperature-sensitive nature of ts045 allows abrupt releaseof the cargo G protein from the ER, enabling morphological characterization of sequential transport intermediates (Plutner et al., 1992). NRK cells were transfected with a ts-G-GFP protein construct(Scales et al., 1997) and held at 40°C to accumulate thecargo in the ER. At 40°C, ts-G-GFP was found to largelycolocalize with calnexin in the ER (Fig. 4, top). It oftenappeared that calnexin was enriched in different sections ofER tubules, whereas the ts-G-GFP was more homogeneously distributed.However, both of these proteins clearly resided in contiguousregions of the same ER tubules. As expected, rbet1 peripheralstructures only partially overlapped with the ER-retained cargo.Fig. 4 (middle) demonstrates that although many rbet1 spotsfall along ER tubules and contain the green cargo, many also lie just adjacent to (see arrows) or even some distance (arrowheads)from the ER structures and lack ts-G-GFP. Hence, it appearsthat cargo in the ER does not have access to a portion of therbet1-containing structures, indicating that sorting and/orvesicle transport is required to move from the ER into thesestructures. A similar relationship is observed between VSV-Gand membrin under these conditions (Fig. 4, bottom, arrows).Before releasing ts-G-VSV from the ER 18% of the rbet1 punctaand 4% of the membrin puncta colocalize with ts-G-VSV.

When released from the ER by shifting to 32°C, the ts-G-GFPcargo quickly began entering peripheral structures distinctfrom the ER. As seen in Fig. 5 (top), after 5 min at the permissivetemperature, the cargo was still very apparent in the ER, butwas also present in calnexin-negative puncta (see arrows).This is similar to those that contained the ER/Golgi SNAREs.5 min after release of cargo from the ER, 57% of rbet1 and27% of membrin puncta colocalized with ts-G-GFP. The cargo becamemore concentrated in these puncta as transport continued. By10 min after release from the ER, the ER staining was weakand the peripheral puncta and Golgi area staining was intense. At this time 42% of rbet1 and 52% of membrin puncta colocalizedwith ts-G-GFP (Fig. 5, rbet1, middle; membrin, bottom), Thedata indicate that these SNARE-containing structures representbona fide intermediates in cargo transport and are suggestiveof a sequential localization, first in rbet1 and later in membrinpuncta. Concentrated cargo colocalized with SNAREs both in fociin close proximity to and some distance away from ER tubules.

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Figure 5 GFP-labeled secretory cargo rapidly enters and accumulates in punctate rbet1- and membrin-containing structures when released from the ER. (Top row) ts-G-GFP–transfected NRK cells grown at 40°C and incubated for 5 min at 32°C were fixed and the subcellular distribution of ts-G-GFP (left) was compared to the calnexin staining pattern (middle). (Middle row) ts-G-GFP–transfected NRK cells grown at 40°C and incubated for 10 min at 32°C were fixed, and the subcellular distribution of ts-G-GFP (left) was compared to the rbet1 staining pattern (middle). (Bottom row) ts-G-GFP–transfected NRK cells grown at 40°C and incubated for 10 min at 32°C were fixed and the subcellular distribution of ts-G-GFP (left) was compared to the membrin staining pattern (middle). Right column respresents an overlay of the previous two images in the row. Arrows and arrowheads point out peripheral rbet1-containing structures that do not appear to overlap ER tubules, yet clearly contain the ts-G-GFP cargo. The arrowheads in the inset point to a structure enriched for both SNAREs and cargo that is clearly distinct from the ER, perhaps representing a mobile VTC en route to the Golgi complex. Bars: (frames) 10 µm; (insets) 4.3 µm.

By 60 min after release from the ER, cargo was visible predominantlyin the Golgi and plasma membrane, with little ER or peripheralIC staining (not shown). Overall the data suggest that thecargo moves from broadly dispersed locations within the ER intothe SNARE-containing peripheral sites where it exits these domainsand travels to the Golgi apparatus.

SNARE-containing Organelles Revealed by Fluorescent Protein Fusions
To better understand the dynamics of transport intermediatescontaining SNARE proteins we transfected cells with variousfluorescent proteins (FPs) fused to either the NH₂- or COOH-terminalends of the SNAREs (Fig. 1). Either stable or transient expressionin NRK cells was used to observe the localization of the SNARE-FPfusion proteins. Consistent with our previous experience, thetransfected SNARE-FPs localized in very similar, if not identical,patterns to those of the endogenous proteins (Fig. 6).

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Figure 6 GFP-tagged SNAREs display a localization, sensitivity to BFA, and 15°C behavior similar to that of the endogenous proteins. Seven SNAREs were fused to GFP and images were captured at 37°C, in the presence of BFA for 1 h, or after 1 h at 15°C. The width of each panel is 56 µm.

In transient expression experiments we examined the SNARE-FPlocalization in cells expressing widely varying levels of thetransfected product based on the fluorescence intensity. Atall intermediate levels of expression the pattern matched closelywith that of the endogenous protein. To further investigatethe dynamics of the GFP-tagged SNAREs compared to the nativeprotein we treated transfected cells with Brefeldin A (BFA)or lowered the temperature to 15°C. Again the GFP-taggedSNARE proteins behaved as the wild-type proteins (Fig. 6).For example, GOS-28 is little effected at 15°C, while membrin,rbet1, and Sec22 become dispersed within the cytoplasm into a punctate distribution. Treatment of syntaxin 13–transfectedcells with BFA resulted in redistribution into a compact spotwhereas the Golgi region staining of sec22b and the other ICSNAREs dispersed into a punctate fluorescence pattern. Thesedata support the notion that the trafficking pathways of thetransfected GFP-tagged SNAREs are very similar if not identicalto the endogenous proteins.

To see if SNARE-FP incorporates into complexes we used antibodiesagainst syntaxin 5 to immunoprecipitate solubilized membranesfrom cells transfected with ER/ Golgi SNARE-FPs. SNARE-FPs werefound to be present in complexes with endogenous proteins. Forexample, immunoprecipitation of endogenous syntaxin 5 resultedin coimmunoprecipitation of membrin-GFP (not shown). Also,GFP mAbs (CLONTECH Laboratories) were able to precipitate endogenoussyntaxin 5 in membrin-GFP– transfected cells but not GFP-transfectedcells. Finally, the presence of GFP-tagged proteins did alterthe localization of other endogenous SNAREs (data not shown).Taken together, these data support the hypothesis that thetransfected SNARE-FPs have many, if not all, of the properties of the endogenous molecules.

To directly test the hypothesis that cargo moves into rsec22b/rbet1peripheral sites and exits these sites, we performed time-lapseimaging of cells transfected with spectrally distinct fluorescentproteins (Fig. 1). We used various fluorescent protein combinationsand found that although GFP and BFP are spectrally distinct,photodamage of BFP led to rapid diminution of the signal making this combination impossible for imaging studies. YFP and CFPare spectrally distinct and also photostable, allowing imagingof both proteins in a single cell. We did not observe any bleedthroughinto the CFP channel in YFP-transfected cells and vice versa.Thus, the CFP-YFP combination of fluorescent proteins is idealfor double-labeled imaging studies. After release of ts-G-YFPfrom the temperature block we observed accumulation of the cargo protein in a preexisting rsec22b-CFP–labeled site (Fig.7, A and B). Subsequently, the colabeled sites lose the ts-G-YFP,leaving behind the rsec22b-CFP (Fig. 7, C and D). The ts-G-YFPdynamics observed are similar to those previously described(Presley et al., 1997; Scales et al., 1997). These data confirmour hypothesis suggesting that the peripheral rsec22b/rbet1-enrichedsites are indeed ER exit sites. We interpret our data as thedirect observation of the filling and exit of cargo from ERexit sites which remain behind at a fixed position within thecell.

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Figure 7 rsec22b sites concentrate cargo that travel to the Golgi complex. (A) rsec22b-CFP labels peripheral sites. Time in minutes:seconds for A and B is indicated. (B) ts-G-YFP is localized in the ER and, upon release from the temperature block, becomes concentrated at preexisting rsec22b-CFP sites. (C) rsec22b-CFP labeling of peripheral sites. Time in minutes:seconds for C and D is indicated. (D) 5 min after release from the temperature block ts-G-GFP is depleted from rsec22b sites. Panel width is 6.2 µm.

The Dynamics of SNARE-FP–labeled Organelles in Living Cells
Many types of organelle movements were observed in the videoimages of living cells transfected with FP-tagged SNAREs. Asummary of movements observed at 3-s intervals with a 1-s exposuretime is shown in Fig. 8. Each type of event is depicted bya particular combination of symbols so that summaries of organellemovements can be presented in later figures. The first typeof movement involves a fluorescent organelle moving in the fieldwithout significant morphological changes (Fig. 8 A). Between0 and 4 s the organelle has moved 3.9 µm and between4 and 8 s the organelle has moved in the same general direction another 2.4 µm. This movement is summarized by a closed circle with an arrow pointing in the direction that the organelleis moving. Since the organelle is observed in the second frameit is again depicted by a circle followed by another arrowthat ends at the position of the organelle in the third frame.We interpret this movement to be a membrane element or clusterof elements maintaining its structure and simply moving fromone position to the next. The rate of this type of movementis $~$ 0.75–1.0 µm/s.

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Figure 8 SNARE-GFP fusions undergo a variety of distinct movements. 1-s exposures are taken with 3 s between exposures. Symbols at the far right are used to represent the class of event. (A) Syntaxin 6-GFP; (B) rsec22b-GFP; (C) rsec22b-GFP; (D) lower magnification of C; (E) rsec22b-GFP; (F) rsec22b-GFP; (G) syntaxin 13-GFP; (H) syntaxin 13-GFP; and (I) rbet1-GFP. The width of a panel is 7.9 microns, except in panel D where the length is 22.2 µm.

A similar movement is observed in Fig. 8 B; however, this timea streak of fluorescence is observed emanating from an organellein frame one and ending at an organelle that appears in framethree. Since the two types of movements (Fig. 8, A and B) maybe mechanistically different we illustrate them slightly differently;in the latter case an open circle is connected to a closedcircle by an arrow pointing in the direction of the movement.A streak of fluorescence may originate from either a structuremoving while the shutter is open, in effect blurring acrossthe CCD array, or from an elongated, tubular organelle. Herewe favor the former case since the structure in the originalposition is not present in the final image and the streak isthe same width as the original organelle.

We also observe streaks emanating from round, $~$ 0.75-µmorganelles. However, in this case the streaks either loosetheir fluorescence or are lost from our field of view in someother fashion (Fig. 8 C). These events are illustrated by aclosed circle at the base of an arrow. In many cases we areable to follow the fluorescent streaks emanating from a spherethrough several frames (Fig. 8 D; left frame is a lower magnificationimage of the region shown in Fig. 8 C, middle frame). We depictthese events by a closed circle with an arrow emanating inthe direction of the streak, as in Fig. 8 C. The subsequentfluorescent streaks are illustrated as arrows (without a circleat the base or the end) pointing in the direction of the movement and proportional to the length of the streak (Fig. 8 D). Ratesof movements seen with this type of event are 1.3 ± 0.7 µm/s. These dynamics we interpret as extending tubulesor vesicle streams because the streaks are thinner than theorganelle from which they originate and at least a fractionof the original organelle remains behind at the initial position.In addition, in images collected with 0.5-s exposure times withno dark time between exposures we see partial overlap in differentexposures along the length of the tubule (not shown). In otherwords, the end of a tubule in one exposure may have moved tothe midpoint of the tubule in the next image.

Another type of movement observed is a streak that ends ina spherical organelle, depicted by an arrow with a closed circleonly at the arrow head (Fig. 8 E). Fluorescent spheres arealso observed to emit a streak that appears to consume thefluorescence of the sphere. This is depicted by an arrow pointingin the direction of the streak with an open circle at the origin(Fig. 8 F). These movements could either be tubules emanatingfrom the sphere or the sphere itself moving while losing fluorescence.Lengths of the arrows are proportional to the distance of themigration during the time interval or the length of the fluorescentstreak.

Post-Golgi SNARE proteins exhibited additional events as illustratedin Fig. 8, G and H. Organelles are observed approaching theplasma membrane followed by an increase in the fluorescencealong the membrane, suggesting an exocytotic membrane fusionevent. Conversely, we observe bright fluorescent regions ofthe membrane followed by the appearance of an intracellularorganelle, which suggests an endocytic event. These events aredepicted by a line along the plasma membrane followed by anarrow pointing either toward (exocytosis), or away (endocytosis) from the plasma membrane. At this level of resolution we cannotrule out the possibility that the organelles are only in closeproximity to the membrane and that we are not observing actualexo- or endocytic events. Finally, using several labeled SNAREswe have observed two organelles that appear to become connectedby a tubule, suggesting the transfer of contents between thestructures. To illustrate these events we connected two circleswith a line (Fig. 8 I).

ER and Golgi SNARE Dynamics
To follow the dynamics of individual organelles and/or transportintermediates labeled with SNARE-FP we imaged cells and plottedthe movements according to the key outlined in Fig. 8. Movementsof SNARE-GFP organelles are shown in Fig. 9, where each colorrepresents the pathway of a separate element plotted at up tonine positions.

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Figure 9 SNARE dynamics. (A) Sec22b-GFP–transfected cell with the pathways of individual organelles illustrated by different colors according to the key in Fig. 8. 1-s exposures were taken every 3 s. (B) rbet1-GFP. (C) syn5-GFP. (D) Membrin-GFP. An asterisk illustrates two structures that appear to associate with each other, whereas an open triangle marks two structures that appear to dissociate from each other. (E) Syntaxin 6-GFP is shown with 0.5-s exposures followed by 2.5 s of dark time. (F) Syntaxin 13-GFP. 0.5-s exposures followed by 1.5 s of dark time. Bars, 5 µm.

rsec22b-GFP and rbet1-GFP are observed at peripheral sites,consistent with our previous observations of a significant contingentof these SNAREs in the ER (Fig. 9, A and B). Peripheral fluorescentsites are most easily observed with rsec22b-GFP and are largelystationary with the exception of some small movements that mightbe due to Brownian motion. Far fewer back and forth movements are observed with rsec22b than with membrin (see below). Importantly,these relatively stationary structures are the points of originof streaks of fluorescence that often travel across the cytoplasmtoward the Golgi region (note the solid line with red, green,and blue traces emanating from a single structure in Fig. 9A). 29% of the movements observed were of this type (C in Fig.8) and 40% of the movements were migrating fluorescent streaks(D in Fig. 8). We hypothesize that these streaks representtubules or closely aligned rows of vesicles carrying cargofrom ER exit sites to the Golgi area. Since distinct streaksemanating from a particular site at different times follow asimilar pathway, the organelles are likely traveling on thesame or parallel microtubule tracks. Other types of rsec22b-GFP movements were as follows: 16% (Fig. 8 A), 10% (Fig. 8 F),and 4% (Fig. 8 I). Relatively little motion is seen in the retrograde direction, suggesting that the recycling of rsec22boccurs via a process that is rare or difficult for us to observe.In the example of a retrograde movement in Fig. 9 A (dashedwhite and purple arrows pointing away from the Golgi region),the site is consumed. While quite similar motions are recordedfor rsec22b-GFP and rbet1-GFP, it was more difficult to followthe rbet1-GFP particles for long distances, perhaps becausethe fluorescence intensity is fainter. We observed a few rbet1-GFPsites near the Golgi region that appear to connect to eachother via tubules (Fig. 9 B).

Syntaxin 5-GFP displays less frequent movement events in ourrecordings. The events observed are similar in character tothe other ER and Golgi SNAREs although fewer long distancemovements from peripheral sites were recorded (Fig. 9 C). Thecell in Fig. 9 D expresses the transfected membrin-GFP fusionprotein at a moderate to low level. Hence, the fainter moreperipheral spotty structures distal to the intermediate compartmentare not readily observed. Interestingly, 100% of the observedmembrin-FP– labeled organelles transit away from and backto the Golgi region (Fig. 8 A). The most intricate of theseis illustrated in yellow where a membrin-FP particle originatesin a region that may be within the Golgi complex, transits out and away from the Golgi complex, wanders, and then returnsto the Golgi region. Other organelles (blue, violet, pink)display similar patterns, moving back and forth between theGolgi region and more peripheral sites. The average rate ofmovement is 0.7 ± 0.3 µm/s. Organelles can beobserved to intersect and form a pair, or to dissociate froma previously existing pair.

We speculate that these movements are antero- and retrogrademovements of vesicles, clusters of vesicles, or small tubulesbetween the ER, IC, and the Golgi apparatus. Interestingly,as a cell enters mitosis the membrin-GFP becomes fragmented,appearing more evenly dispersed about the cell (data not shown).Furthermore, organelle movements cease or are dramaticallyreduced, which is consistent with the previously describedchange in secretory events associated with mitotic cells (Warren et al., 1995).GOS28-GFP shows few if any detectable events on the time scalewe recorded from the transfected cells (data not shown). Thisbehavior of GOS28 is consistent with our previous observationsthat the protein changes little upon a temperature shift to15°C and that GOS28 appears to be in distinct complexesfrom the other ER to Golgi SNAREs (Hay et al., 1998).

We also studied the dynamics of two post-TGN SNARE proteins,syntaxin 6-GFP and syntaxin 13-GFP (Fig. 9, E and F). The movementsrecorded for syntaxin 6-GFP are very unique as they are allof the type illustrated in Fig. 8 A, that is, spherical organellesmigrating within the cell. A single organelle was traced through11 frames illustrating movements towards, away from, and parallelto the TGN (Fig. 9 E, pink solid line). Syntaxin 6-GFP–labeledorganelles can also be seen to reverse direction abruptly. In contrast to syntaxin 6-GFP, syntaxin 13-GFP–labeled organellesexhibit a wider variety of movements. Movements of sphericalorganelles as well as tubules are documented in Fig. 9 F. Inaddition, we observe syntaxin 13-GFP organelles that approachthe plasma membrane, possibly fusing, and events that havethe appearance of endocytosis (Fig. 8, G and H). Directionsof the syntaxin 6 and 13-GFP movements are much more randomin orientation than those of rsec22b-GFP and membrin-GFP.

To follow the movements of multiple SNAREs in a single cellwe again used the YFP, CFP combination of fluorescent proteins.rsec22b-CFP coexpressed with membrin-YFP exhibits a higherdegree of colocalization when compared to rsec22b-CFP coexpressedwith syntaxin 13-YFP. However in the rsec22b-CFP/membrin-YFPcotransfected cells, the ratios of the two SNARE-FPs are notalways equal because some organelles appear to contain moreof one SNARE while other organelles contain more of the other (Fig. 10, A–C). This observation is consistent with thedifferent overall dynamics observed for the two SNAREs. Withthis technique we are further able to observe the following:some membrin and rsec22b movements are distinct, and in somecases the colabeled rsec22b and membrin sites move synchronously.

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Figure 10 Overlapping and distinct SNARE trafficking pathways. Cotransfection of (A) rsec22b-CFP and (B) membrin-YFP reveals colocalizing structures (double arrow) and structures containing mostly membrin (arrowhead) or rsec22b (arrow). (C) A and B merged image. Moving structures that contain rsec22b and membrin appear as a double (yellow and cyan) spot because of the 1.25-s time difference between the exposures. Bars, 5 µm.

	Discussion

Top Abstract Materials and Methods Results Discussion References

We have studied the organization of the secretory pathway byfusing fluorescent proteins to VSV-G, a widely utilized cargoprotein, and SNAREs, molecules important for membrane fusion.By following the dynamic movements of organelles labeled withthese reagents we are able to better understand the mechanismswhereby proteins are translocated through the secretory pathway. Since SNARE proteins are critical determinants of an organelle'sidentity, these proteins serve as specific labels of functionalcompartments. Beginning at the ER, several interesting observationsemerged from this work. At 40°C the ts-G-GFP is retainedin the ER where the staining is similar to both calnexin andBip. Many of the SNARE-labeled structures are closely juxtaposedto the ER, as if they lie alongside the tubules of the organelle.When the temperature of the transfected cells is lowered, allowing the VSV-G to flow through the secretory pathway, the proteinaccumulates in the 0.75–1-µm structures that preciselyoverlap with SNAREs at sites we believe to be the positionof exit from the ER.

Double labeling with SNAREs and cargo reveals that rsec22bprecedes cargo at these ER sites. The theory that these structuresare ER exit sites is further confirmed by the dynamics of fluorescentSNARE proteins, particularly rsec22b-GFP. We observe streaksof fluorescence emanating from these sites that we interpretto be tubules or rows of closely spaced vesicles. Multiplestreaks are commonly observed to emanate sequentially froma single exit site that suggests the ER exit sites are usedmultiple times. Their direction of transport is most oftentoward the Golgi region (suggesting anterograde trafficking)and sequential streaks follow similar paths along what arelikely to be the same or closely aligned microtubules. Thispicture is somewhat different than that observed for the real-timedynamics of cargo, where the peripheral structures were notedto move toward the Golgi complex (Presley et al., 1997).

In contrast, our data support the view of a fixed ER exit sitethat serves to load transport organelles (vesicles or emergingtubules) with cargo while sorting ER proteins in a retrogradefashion back to the ER. When the transport vesicles or nascenttubules have matured, we propose that they translocate to theGolgi apparatus along microtubules and a new round of cargoloading and protein sorting initiates at the same site. Nevertheless,the regulation of membrane dynamics at these ER exit sitesneeds to be further investigated. For example, it would beimportant to learn what accounts for the apparently sporadicnature of the fluorescent streaks; perhaps they signify cargoexport. In addition, it is of interest to know whether thereis a functional difference between the SNARE-labeled sites that appear to colocalize with ER markers (perhaps in segmentsof ER tubules) and those puncta that exclude ER markers andlie directly alongside or some distance from ER tubules. Also,it is not yet known how SNAREs concentrate at certain siteswhile excluding resident ER proteins.

Interestingly, membrin, a SNARE proposed to function in concertwith rsec22b through the formation of complexes (Hay et al., 1998)and whose still-life localization significantly overlaps thatof rsec22b, appears to display significantly different dynamicsthan rsec22b. Membrin appears to reside on mobile $~$ 1-µmorganelles that themselves move between the cis-Golgi regionand more peripheral sites. On the other hand, while rsec22bis more apparent on stationary, peripheral, $~$ 1-µm structuresfrom which steaks of fluorescence emanate, generally toward the Golgi region. One possibility is that rsec22b and rbet1 are more enriched in small transport vesicles/tubules that stream outward from larger foci. This would be consistent with the EM study that found a larger percentage of rsec22band rbet1 vesicles also contained COPII when compared to syntaxin5– or membrin-containing vesicles (Hay et al., 1998).The mobile 1-µm structures containing membrin may containrsec22b and rbet1 as well, but these SNAREs may be more vigorouslysorted away when these structures are translocated. This hypothesismight explain why the movements shown in Fig. 8 A appear rarerthan those shown in Fig. 8 F, which are more common in the movies of rsec22b- and rbet1-FPs. What is the function of the mobile 1-µm structures? Perhaps they function as anterogradeand/or retrograde transport organelles in conjunction with smallER-derived vesicles. The small vesicles/tubules may serve tofill the membrin-enriched larger structures which then actas carriers in and out of the Golgi area. These organellescould then be thought of as mobile extensions of the cis-Golginetwork.

Since the fluorescence of syntaxin 5–transfected cells was not as bright as rsec22b, we may not have detected particularclasses of movements. Given this caveat, syntaxin 5 dynamicswere generally the same types as the other mobile ER and GolgiSNAREs; however, movements were less frequent, perhaps reflectinga less dynamic nature of this SNARE. The tubular extensionsobserved between organelles (see Fig. 8 I) may be conduits for the transfer of cargo between organelles. Alternatively,these structures may represent transport tubules that fusewith the acceptor compartment before fission from the donorcompartment.

The dynamics of the two post-Golgi SNAREs, syntaxin 6 and syntaxin13, were very different from the ER-to-Golgi proteins. Syntaxin6 localizes largely to the TGN, and less so to endosomes. Syntaxin6-FP appears on organelles that meander through the cytoplasm,some of which travel away from the Golgi region, reverse direction,and travel back toward this site again, perhaps reflecting cyclingbetween the TGN and endosomes. The precise nature of any cargocontained in these organelles remains unknown. However, thelocalization and dynamics are consistent with a role in TGNto endosome trafficking. Syntaxin 13 is proposed to representa SNARE in the plasma membrane/recycling endosome pathway (Prekeris et al., 1998;Tang et al., 1998). Consistent with this proposal, syntaxin13-FP labels were the only organelles we were able to observein potential plasma membrane fusion and recycling events. Inaddition, the dynamics appear to reveal tubules that extendfrom a central organelle. Perhaps these tubules, formed as proteins,are sorted within the early endosome.

The most remarkable feature of cellular dynamics reinforcedby these studies is the specificity of the multitude of traffickingevents. The direction and mode of movements, the size and shapeof the organelles, and the destinations of the organelles areall precisely regulated. These events are likely to be thecritical determinants of the specificity of vesicle traffickingand the membrane organization of cells. Clearly when an organellearrives at its appropriate destination within the cell an adequatemachinery, likely comprised of SNAREs, must catalyze the membranefusion events. But how cargo and SNAREs are specifically coupledto the organelle translocation machinery, likely comprisedof motors and cytoskeletal tracks, remains unclear. Recent reportsof motor proteins binding specific Rab proteins may be partof the solution to the molecular recognition issues that underliethis problem. Perhaps purification of the SNARE-FP–taggedorganelles will help lead to a solution to this problem.

Acknowledgments

The authors thank Dr. Suzanne R. Pfeffer for her efforts inestablishing the Stanford University Cell Sciences ImagingFacility; Dr. Susan L. Palmieri for her excellent managementof the facility; Dr. Carolyn Machamer (The Johns Hopkins University)for permission to use VSV-G-ts045; Dr. Suzie Scales for technicaladvice regarding VSV-G-ts045; and Paul Millman of Chroma TechnologyCorporation for technical expertise regarding fluorescent proteinoptical equipment. We also thank rotation students Mr. IgorBrodsky and Ms. Grace Park for help in making some of the constructsused in this work, and Viola Oorschot (Utrecht University) for preparing the ultrathin cryosections.

Submitted: 31 August 1998

Revised: 16 December 1998

Address correspondence to Richard H. Scheller Howard HughesMedical Institute, Department of Molecular and Cellular Physiology,Stanford, CA 94305-5428. Tel.: (650) 723-9075. Fax: (650) 725-4436.E-mail: scheller{at}cmgm.stanford.edu

J.C. Hay's present address is Department of Biology, Universityof Michigan, 830 North University, Room 3065C, Ann Arbor, MI48109-1048.

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