Morphology and Dynamics of Clathrin/GGA1-coated Carriers Budding from the Trans-Golgi Network

doi:10.1091/mbc.02-07-0109

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

Originally published as MBC in Press, 10.1091/mbc.02-07-0109 on January 26, 2003

This Article

	Abstract
	Full Text (PDF)
	Supplemental Videos
	All Versions of this Article: 02-07-0109v1 14/4/1545 most recent
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager


Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Puertollano, R.
	Articles by Bonifacino, J. S.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Puertollano, R.
	Articles by Bonifacino, J. S.

Vol. 14, Issue 4, 1545-1557, April 2003

Morphology and Dynamics of Clathrin/GGA1-coated Carriers Budding from the Trans-Golgi Network

Rosa Puertollano,^* Nicole N. van der Wel, Lois E. Greene, Evan Eisenberg, Peter J. Peters, and Juan S. Bonifacino^*^§

^*Cell Biology and Metabolism Branch, National Institute of Child Health and Human Development and Laboratory of Cell Biology, National Heart, Lung, and Blood Institute, National Institutes of Health, Bethesda, Maryland 20892; and Division of Tumor Biology, The Netherlands Cancer Institute, Amsterdam, The Netherlands

Submitted July 15, 2002; Revised October 22, 2002; Accepted December 4, 2002
Monitoring Editor: Suzanne R. Pfeffer

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Sorting of transmembrane proteins and their ligands at various compartments of the endocytic and secretory pathways is mediatedby selective incorporation into clathrin-coated intermediates.Previous morphological and biochemical studies have shown thatthese clathrin-coated intermediates consist of spherical vesicleswith a diameter of 60-100 nm. Herein, we report the use of fluorescentimaging of live cells to demonstrate the existence of a differenttype of transport intermediate containing associated clathrincoats. Clathrin and the adaptors GGA1 and adaptor protein-1, labeledwith different spectral variants of the green fluorescent protein,are shown to colocalize to the trans-Golgi network and to a populationof vesicles and tubules budding from it. These intermediates arehighly pleiomorphic and move toward the peripheral cytoplasm fordistances of up to 10 µm with average speeds of ~1 µm/s. The labeledclathrin and GGA1 cycle on and off membranes with half-times of10-20 s, independently of vesicle budding. Our observations indicatethe existence of a novel type of trans-Golgi network-derived carrierscontaining associated clathrin, GGA1 and adaptor protein-1 thatare larger than conventional clathrin-coated vesicles, and thatundergo long-range translocation in the cytoplasm before losingtheircoats.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Clathrin coats associated with the cytosolic face of membranes mediate the sorting of transmembrane proteins and their boundligands at the plasma membrane, the trans-Golgi network (TGN)and endosomes (Kirchhausen, 2000; Brodsky et al., 2001). The majorbuilding blocks of clathrin coats are clathrin triskelia composedof three heavy chains and three light chains (a or b isoforms),which assemble into polyhedral lattices. At each intracellularlocation, clathrin coats contain a characteristic set of heterotetramericadaptor protein (AP) complexes that mediate both attachment ofthe clathrin lattices to membranes and concentration of specifictransmembrane proteins. The AP-2 complex plays such roles at theplasma membrane, whereas the AP-1 complex does so at the TGN and/orendosomes (Kirchhausen, 2000; Brodsky et al., 2001; Robinson andBonifacino, 2001). Recently, a family of monomeric proteins termedGGAs (i.e., GGA1, GGA2, and GGA3 in humans) has also been shownto promote recruitment of clathrin and sorting of transmembraneproteins at the TGN (Robinson and Bonifacino, 2001; Boman, 2001).In particular, the GGAs have been implicated in the sorting thecation-dependent and cation-independent mannose 6-phosphate receptors(CD- and CI-MPRs, respectively) from the TGN to the endosomal-lysosomalsystem (Puertollano et al., 2001a; Takatsu et al., 2001; Zhu etal., 2001). This sorting is mediated by interaction of the amino-terminalVHS domain of the GGAs and acidic-cluster-dileucine sorting signalspresent in the cytoplasmic domains of the MPRs (Puertollano etal., 2001a; Takatsu et al., 2001; Zhu et al., 2001). The VHS domainof the GGAs has also been shown to interact with acidic-cluster-dileucinesignals in the cytoplasmic domains of other transmembrane proteinssuch as sortilin (Nielsen et al., 2001), the low-density lipoproteinreceptor-related protein 3 (Takatsu et al., 2001), and $beta$ -secretase(He et al., 2002), all of which may also cycle between the TGNandendosomes.

Despite recent advances in the elucidation of the role of the GGAs in protein sorting, many outstanding issues remain concerning1) whether the GGAs colocalize with clathrin and AP-1 on transportintermediates budding from the TGN, 2) the morphology of theseGGA-containing intermediates, 3) the intracellular destinationof these carriers, and 4) the dynamics of GGA cycling on and offTGN membranes in vivo. These issues have recently become amenableto analysis through the use of fluorescence imaging technologieson live cells. The dynamics of plasma membrane clathrin-coatedpits, for example, have been examined using clathrin constructstagged with variants of the green fluorescent protein (GFP) (Gaidarovet al., 1999; Damer and O'Halloran, 2000; Wu et al., 2001). Thisapproach revealed that clathrin-coated vesicles (CCVs) emanaterepeatedly from the same sites, suggesting the existence of "hot-spots"for CCV formation from the plasma membrane (Gaidarov et al., 1999).The same approach was used to demonstrate a rapid (t_1/2 ~16 s),ATP-dependent exchange of clathrin triskelia on plasma membranecoated pits, which may allow remodeling of the coat as the membraneinvaginates (Wu et al., 2001). Strikingly, clathrin exchange onthe pits occurs even when endocytosis is blocked (Wu et al., 2001),indicating that the coats are not static assemblies and that uncoatingdoes not require vesicle detachment from the membrane. To date,the characteristics of protein coats associated with the TGN inliving cells remain to be similarlyexamined.

Herein, we report the results of a study on the morphology and dynamics of GGA1-, AP-1-, and clathrin-coated structures atthe TGN in vivo. By using GGA1, the $gamma$ 1 subunit of AP-1, and clathrinlight chain b isoform labeled with different spectral variantsof GFP, we show that all of these coat proteins colocalize tothe TGN and to a population of vesicular-tubular carriers buddingfrom the TGN. Surprisingly, these carriers are pleiomorphic andapparently larger than conventional CCVs. They move centrifugallyfor distances of up to 10 µm and with average speeds of 1 µm/s.The fluorescently labeled clathrin and GGA1 constructs cycle onand off membranes with t_1/2 of 10-20 s. This cycling is not dependenton budding from the TGN, suggesting that assembly and disassemblyof the coats can be functionally uncoupled from vesicle budding.These results suggest the existence of a novel type of TGN-derivedcarriers containing associated clathrin that are larger and moredynamic than conventional CCVs, and that undergo long-range translocationin the cytoplasm before losing theircoat.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Recombinant DNA Procedures and Antibodies

A cDNA encoding full-length human GGA1 was cloned into the SalI and BamHI sites of the pEGFP-C1, pEYFP-C1, and pECFP-C1 vectors(BD Biosciences Clontech, Palo Alto, CA). Clathrin light chainb was amplified from human placenta Quick-Clone cDNA (BD BiosciencesClontech) and cloned into the pEYFP-C2 vector via EcoRI and SalIsites. Plasmids encoding cyan fluorescent protein (CFP)-vesicularstomatitis virus G (VSV-G) (ts045 mutant) and CFP-galactosyl transferasewere the kind gift of Jennifer Lippincott-Schwartz (National Instituteof Child Health and Human Development). The cloning of the Myc-epitope-taggedGGA1 and CD-MPR-CFP was described previously (Dell'Angelica etal., 2000; Puertollano et al., 2001a).

The following commercial antibodies were used: mouse monoclonal and rabbit polyclonal anti-myc antibodies (9E10; Covance,Princeton, NJ), mouse monoclonal antibody to $gamma$ 1-adaptin (100/3,Sigma-Aldrich, St. Louis, MO), and mouse monoclonal antibody toclathrin (CHC; Transduction Laboratories, Lexington, KY). Thepreparation of rabbit polyclonal antibody to AP-3 ( $beta$ 3C1) has beendescribed in a previous report (Dell'Angelica et al., 2000). Apolyclonal antibody to GGA1 was the kind gift of Margaret S. Robinson(University of Cambridge, Cambridge, UnitedKingdom).

Immunofluorescence Microscopy

Nonpolarized Madin-Darby canine kidney (MDCK) cells were grown on coverslips and fixed in methanol/acetone (1:1, vol/vol)for 10 min at $-$ 20°C and subsequently air-dried. Incubation withprimary antibodies diluted in phosphate-buffered saline (PBS),0.1% (wt/vol) saponin, 0.1% bovine serum albumin, was carriedout for 1 h at room temperature. Unbound antibodies were removedby rinsing with phosphate-buffered saline for 5 min, and cellswere subsequently incubated with secondary antibodies (Cy3-conjugateddonkey anti-rabbit Ig and Alexa 448-conjugated donkey anti-mouseIg) diluted in PBS, 0.1% (wt/vol) saponin, 0.1% bovine serum albumin,for 30-60 min at room temperature. After a final rinse with PBS,coverslips were mounted onto glass slides with Fluoromount G (SouthernBiotechnology Associates, Birmingham, AL). Fluorescence imageswere acquired on an LSM 410 or LSM 510 confocal microscope (CarlZeiss, Thornwood,NY).

Immunoelectron Microscopy

Cryogold immunoelectron microscopy of monocyte-derived dendritic cells and stably transfected MDCK cells was performed asdescribed previously (Porcelli et al., 1992; Peters, 1998)

Fluorescent Imaging of Living Cells

MDCK cells were grown on LabTek chambers (Nalge Nunc, Naperville, IL), transfected with different constructs tagged with GFPspectral variants by using FuGENE 6 (Roche Diagnostics, Indianapolis,IN), and transferred into culture medium buffered with 25 mM HEPES/KOHpH 7.4. Experiments were performed using an inverted confocallaser scanning microscope (LSM 510; Carl Zeiss) equipped witha stage heated to 37°C. argon, HeNe, and krypton lasers; and a63× 1.4 numerical aperture objective. Yellow fluorescent protein(YFP) and CFP fluorescence were visualized using excitation filtersat 514 and 413 nm and emission filters at 530 and 515-430 nm,respectively, whereas GFP was excited with a 488-nm filter andimaged through a 515- to 545-nm emission filter. When indicated,endosomes were loaded with rhodamine-conjugated human serum albuminor rhodamine-conjugated transferrin (Molecular Probes, Eugene,OR), which were imaged using a 543-nm laser. Cells expressingCFP-VSV-G (ts045 mutant) were cultured at 40°C for 24 h, shiftedto 20°C for 1 h, and then to 32°C before visualization. Imageswere recorded every 3 or 6 s. To estimate the size of GGA1-coatedintermediaries, MDCK cells expressing YFP-GGA1 were incubatedwith medium containing yellow-green fluorescent beads (FluoSpherescarboxylate-modified microspheres, 2.0 µm; Molecular Probes) andanalyzed by time-lapse confocal microscopy as described previously.Data were processed to QuickTime format in Adobe Premiere 5.0.

Photobleaching was performed at high laser power (100% power, 100% transmission). Recovery was followed by scanning the wholecell at lower power (40%) and attenuated transmission (3%) atintervals from 5 s to 5 min. A nearby background region of equalarea was similarly measured and subtracted. Background pixel valueswere <20% of the average intensity of these structures. Fluorescenceintensity was normalized to the first timepoint.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Distribution of Coat Proteins Associated with TGN in MDCK Cells

We chose to perform our imaging studies on nonpolarized MDCK epithelial cells because they 1) are large and flat, 2) havean extensive TGN, and 3) yield low-to-moderate expression of constructsdriven from the human cytomegalovirus promoter, as is the casefor the plasmid vectors used herein. The use of MDCK cells, however,necessitated a reexamination of the distribution of various coatproteins associated with the TGN, as previously established forother cell lines. We started by performing immunofluorescencemicroscopy of MDCK cells stably transfected with a Myc-taggedGGA1 construct (Myc-GGA1). Immunoblot analyses with an antibodyto GGA1 revealed that the expression levels of Myc-GGA1 were four-to fivefold higher than those of endogenous GGA1 (our unpublisheddata). Consistent with previous findings in other cell lines (Hirstet al., 2001; Puertollano et al., 2001b), we observed extensivecolocalization of Myc-GGA1 with clathrin in the area of the TGN(Figure 1, A-C). We also observed considerable overlap of Myc-GGA1and AP-1 staining at the TGN (Figure 1, D-F). Outside the TGN,Myc-GGA1, AP-1, and clathrin displayed various degrees of colocalizationto cytoplasmic structures having apparent diameters of ~400 nm(Figure 1, insets). Quantification of these results showed thatalmost 100% of all resolvable GGA1-containing foci colocalizedwith clathrin (148 foci counted), whereas 40% colocalized withAP-1 (110 foci counted). Another AP complex, AP-3, was more peripherallydistributed than either GGA1 or AP-1 and therefore exhibited substantiallyless colocalization with Myc-GGA1 in the area of the TGN (Figure1, G-I). Some peripheral foci, however, seemed to contain bothAP-3 and Myc-GGA1 (Figure 1, G-I, inset).

View larger version (165K):
[in this window]
[in a new window]

Figure 1. Intracellular distribution of Myc-GGA1 in MDCK cells analyzed by immunofluorescence microscopy. MDCK cells stably expressing Myc-GGA1 were fixed, permeabilized, and double labeled by incubation with antibodies to GGA1 (A, red channel), the Myc epitope (D, red channel; G, green channel), clathrin (B, green channel), the $gamma$ 1-adaptin subunit of AP-1 (E, green channel), and the $beta$ 3A subunit of the AP-3 complex (H, red channel), as indicated in the figure, followed by the corresponding fluorescently conjugated secondary antibodies. Stained cells were examined by confocal fluorescence microscopy. Merging the images in the red and green channels generated the third picture on each row (C, F, and I); yellow indicates overlapping localization. Insets show twofold-magnified views of peripheral cytoplasmic regions. Bar, 10 µm.

Immunoelectron microscopy of monocyte-derived dendritic cells, in which endogenous GGA1 can be more easily detected, revealedlocalization of endogenous GGA1 to coated buds with diametersof 60-130 nm in the area of the TGN (Figure 2A), as well as inthe peripheral cytoplasm (our unpublished data). A similar localizationwas observed for Myc-GGA1 in stably transfected MDCK cells (Figure2, B-D). Many coated buds were found to contain both Myc-GGA1and clathrin (Figure 2B, open arrowheads). We also observed partialcolocalization of Myc-GGA1 and AP-1 on coated buds with diametersof 60-130 nm at both the TGN (Figure 2, C-D, open arrowheads)and the cell periphery (Figure 2D, open arrowheads). However,some individual buds contained gold particles labeling only Myc-GGA1or AP-1 (Figure 2, C and D). We detected some gold labeling forall of these coat proteins in the cytosol, consistent with thefact that they cycle between membranes and the cytosol. Buds containingthese coat proteins often occurred in mixed clusters, which mightcorrespond to the larger peripheral structures observed by fluorescencemicroscopy.

View larger version (140K):
[in this window]
[in a new window]

Figure 2. Immunoelectron microscopy localization of GGA1, Myc-GGA1, clathrin and AP-1. (A) Localization of endogenous GGA1 in monocyte-derived dendritic cells was analyzed by cryoimmunogold electron microscopy using antibodies to GGA1 (10-nm gold). (B-D) MDCK cells stably expressing Myc-GGA1 were analyzed by cryoimmunogold electron microscopy using antibodies to the Myc epitope (15-nm gold) and clathrin (10-nm gold) (B), GGA1 (15-nm gold) and the $gamma$ 1 subunit of AP-1 (10-nm gold) (C and D). Open arrowheads in B indicate coated buds containing both Myc-GGA1 and clathrin, whereas closed arrowheads point to 15-nm gold particles marking the location of Myc-GGA1. Open arrowheads in C and D point to coated buds containing both Myc-GGA1 (or GGA1) and AP-1, whereas closed arrowheads point to 15-nm gold particles marking the location of Myc-GGA1 (or GGA1). G, Golgi complex; n, nucleus; p, plasma membrane; m, mitochondrion. Bars, 200 nm.

Characteristics of Coated Carriers Budding from TGN

To examine the morphology and dynamics of coated carrier vesicles budding from the TGN, we constructed plasmids encoding variousspectral variants of GFP attached to clathrin light chain b isoform,GGA1 and the $gamma$ 1-adaptin subunit of AP-1. These proteins were expressedby transfection into MDCK cells. At low-to-moderate levels ofexpression, all three GFP-tagged proteins localized to both juxtanuclearand peripheral structures (Figure 3, A-C), similar to those shownin Figure 1. Time-lapse confocal microscopy of live cells expressingeach of these GFP-tagged constructs revealed that some of theperipheral foci were relatively static (arrowheads), whereas othersmoved rapidly from the TGN toward the peripheral cytoplasm (arrows)(Figure 3, A-C). The structures emanating from the TGN were relativelylarge (360- to 380-nm average diameters; Table 1) in comparisonwith plasma membrane clathrin-coated pits (Gaidarov et al., 1999;Wu et al., 2001). This difference could be readily appreciatedin fields where the larger TGN-derived, clathrin-coated intermediatesmoved in relation to smaller, less mobile clathrin-coated pitsat the cell edges (Figure 3D, size comparison shown in the insets).In addition, the intermediates seemed larger than 200-nm-diameterfluorescent beads of similar brightness added to the cell culturesbefore imaging (Figure 4A, compare fluorescent beads in the insetswith moving intermediate indicated by arrow).

View larger version (142K):
[in this window]
[in a new window]

Figure 3. Characterization of TGN-derived carriers containing clathrin, GGA1, and AP-1. MDCK cells were grown on LabTek chambers and transiently transfected with constructs encoding GFP-clathrin light chain b (A and D), GFP-GGA1 (B), or GFP- $gamma$ 1-adaptin (GFP-AP-1; C). At 15 h after transfection, cells expressing moderate levels of the fluorescent proteins were analyzed by time-lapse microscopy and images acquired at the indicated intervals. Insets in D show twofold-magnified comparisons of clathrin-containing carriers budding from the TGN with clathrin-coated pits at the plasma membrane. Arrows point to pleiomorphic carriers budding from the TGN and moving toward the cell periphery, whereas arrowheads indicate immobile structures. N, nucleus. Bars, 5 µm (A-C), 4 µm (D), 1 µm (D insets). QuickTime videos of the experiments shown in A, B, and C can be seen in Supplemental Materials (videos 1, 2, and 3, respectively).

View this table:
[in this window]
[in a new window]

Table 1. Quantification of the size of foci containing fluorescently labeled clathrin and GGA1

View larger version (48K):
[in this window]
[in a new window]

Figure 4. Comparison of the size of GGA1-coated intermediaries to that of fluorescent beads. MDCK cells expressing YFP-GGA1 were incubated with 0.2-µm-diameter fluorescent beads before analysis by time-lapse confocal microscopy. Arrow in A points to a YFP-GGA1-containing intermediate moving from the TGN toward the cell periphery. Notice that this carrier seems larger (~0.35 µm) than the beads shown in the inset (~0.2 µm), even though these structures have similar fluorescent intensities (37.7 and 38.6 arbitrary units, respectively). In some cases, large intermediates seem to arise from clustering of smaller vesicles, as shown in B (fluorescent bead is shown in the inset). Bars, 0.5 µm (A), 1 µm (B).

The TGN-derived intermediates decorated with any of the three GFP-fusion proteins were pleiomorphic. Most were spheroidalor ellipsoidal. Some detached from the TGN as single vesicles,whereas others pulled off in groups resembling beads on a string(e.g., Figures 3C, 6A, and 7, A and B). They often changed shapesand some even divided during transport (Figure 5B, arrow between6 and 9 s). Others joined or fused during transport, generatingstructures that were bigger and brighter than the original vesicles(Figure 4B).

View larger version (96K):
[in this window]
[in a new window]

Figure 5. Presence of clathrin and AP-1 on GGA1-containing carriers. MDCK cells were simultaneously transfected with constructs encoding YFP-clathrin and CFP-GGA1 (A) or GFP- $gamma$ 1 (GFP-AP-1) and CFP-GGA1 (B). Confocal microscopy images were acquired every 3 s. Arrows indicate vesicular carriers budding from the TGN, whereas arrowheads point to immobile structures. The yellow color in the merged images indicates colocalization between clathrin and GGA1 (A) or GGA1 and AP-1 (B). Bars, 2 µm.

The TGN-derived intermediates moved centrifugally with average speeds of ~1 µm/s. Their trajectories were quasilinear, asif they were tethered to a system of radial tracks. Treatmentwith the microtubule-depolymerizing agent, nocodazole, abolishedthe long-range translocation of the TGN-derived intermediates(our unpublished data), suggesting that movement occurred alongmicrotubules.

Coexpression of combinations of coat proteins, each tagged with a different GFP variant, allowed us to analyze for their presenceon the same coated intermediates. We observed that most TGN-derivedintermediates contained both clathrin and GGA1 (an example isshown in Figure 5A). We could also observe budding of intermediatesthat contained both GGA1 and AP-1 (Figure 5B).

As previously shown (Puertollano et al., 2001a), tubules and vesicles carrying the CD-MPR from the TGN almost always exhibitedassociated GGA1. In the example shown in Figure 6A, a string ofGGA1-containing structures can be seen decorating in discontinuousmanner a CD-MPR-carrying tubule. We occasionally saw endosomalrecycling tubules labeled with internalized rhodamine-transferrinpulling off the juxtanuclear area of the cell, but these almostnever contained associated GGA1 (Figure 6B). Although GGA1- andAP-1-containing intermediates detached and moved away from theTGN, the Golgi resident enzyme galactosyl transferase stayed behindin the Golgi complex (Figure 7, A and B). GGA1-containing intermediateswere distinct from post-Golgi carriers (i.e., PGCs; Hirschberget al., 1998; Polishchuk et al., 2000) that transport the VSV-Gprotein to the plasma membrane (Figure 7C). These observationsillustrate the occurrence of protein sorting at the TGN by generationof distinct types of vesicular carriers.

View larger version (142K):
[in this window]
[in a new window]

Figure 6. Cargo specificity of GGA1-containing intermediates. (A) Confocal microscopy imaging of live MDCK cells coexpressing CD-MPR-CFP and YFP-GGA1. Images were collected at 6-s intervals. Arrows indicate the formation and detachment of long tubular structures containing CD-MPR-CFP from the TGN. Notice that YFP-GGA1 associates with those tubular structures in a discontinuous pattern. (B) MDCK cells expressing GFP-GGA1 were incubated with rhodamine-transferrin for 20 min to load recycling endosomes and then examined by video microscopy. Images show that transferrin-containing intermediates in transit from the juxtanuclear area of the cell are devoid of GFP-GGA1. Bars, 3 µm.

View larger version (90K):
[in this window]
[in a new window]

Figure 7. Exclusion of galactosyl transferase and VSV-G protein from GGA1 carriers budding from the TGN. (A and B) Golgi-resident protein galactosyl transferase (GT) is not incorporated into vesicular carriers budding from the TGN. MDCK cells were doubly transfected with a trans-Golgi resident protein (CFP-GT) and with YFP-GGA1 (A) or GFP- $gamma$ 1 (GFP-AP-1) (B). Time-lapse microscopy showed the absence of CFP-GT (red channel) from rows of coated intermediates budding from the TGN (green channel, arrows). (C) VSV-G and GGA-1 localize to different transport intermediaries. MDCK cells, transfected with YFP-GGA1 and CFP-VSV-G (ts045 mutant) were incubated for 24 h at 40°C, shifted to 20°C for 1 h to accumulate cargo in the TGN, and then warmed to 32°C before visualization. Consecutive video images from time-lapse series show a VSV-G-enriched vesicle budding from the TGN (arrow, red channel). Note the absence of GGA1 (green channel) in this structure. The arrowhead points to a row of YFP-GGA1-containing vesicles rapidly budding from the TGN. N, nucleus. Bars, 10 µm (A and B), 5 µm (C).

Interaction of GGA1-containing Carriers with Endosomes

On arrival at the cell periphery, the fluorescent signal of most TGN-derived, GGA1-containing carriers was lost, perhaps dueto uncoating or movement outside the plane of focus. This preventedus from establishing the final destination of these carriers.Some GGA1-containing structures, however, were found to interactwith endosomes labeled by internalization of rhodamine-albuminfor 15 min. Figure 8 shows an example of such interactions. Inthis example, a GFP-GGA1-coated carrier (green) and a rhodamine-albumin-containing endosome (red) converge to form a single hybrid organelle(yellow). The two markers remain associated with the same structureand move together for 51 s, although at times they seem segregatedto different domains of the hybrid organelle. This structure eventuallyundergoes uneven fission into a vesicle that contains both GGA1and albumin and another vesicle that contains only GGA1. The latterfinally disappears, likely due to uncoating. We have observedvariations on this phenomenon. Sometimes the GFP-GGA1 fluorescenceis quickly lost after the two vesicles merge. Other times theGGA1- and albumin-containing vesicles interact transiently andthen part ways, reminiscent of "kiss-and-run" interactions (Storrieand Desjardins, 1996). We interpret that these events representthe transfer of cargo from the TGN-derived carriers to the endosomalsystem.

View larger version (181K):
[in this window]
[in a new window]

Figure 8. Interaction of GGA1-containing carriers with endosomes. MDCK cells were transfected with GFP-GGA1. At 15 h after transfection, the cells were loaded with rhodamine-albumin for 15 min before analysis by time-lapse confocal microscopy. Merged images for GFP-GGA1 (green) and rhodamine-albumin (red) are shown. Arrows point to vesicular structures containing rhodamine-albumin and GFP-GGA1. The insets show fourfold magnification of the structures pointed by the arrows. Bars, 2 and 0.5 µm (inset).

Dynamics of Clathrin and GGA1 Coats

The ability to visualize fluorescently tagged clathrin and GGA1 in association with the TGN allowed us to examine the ratesof exchange of these proteins between membranes and the cytosolby using the technique of fluorescence recovery after photobleaching(Jacobson et al., 1976). This was performed by photobleachinga region of the TGN and quantifying the time course of fluorescencerecovery in that region. We found that both GFP-clathrin (Figure9A) and GFP-GGA1 fluorescence (Figure 9B) recovered with exponentialkinetics and t_1/2 of ~20 and 10 s, respectively (Figure 9D). Theserates were within the range previously reported for clathrin atthe plasma membrane (Wu et al., 2001) and COPI on the Golgi complex(Presley et al., 2002). Hence, the association of all of theseproteins' coats with membranes is a highly dynamic process. Therecovery seemed to occur on the same structures that were photobleached(Figure 9C, arrows).

View larger version (59K):
[in this window]
[in a new window]

Figure 9. Dynamics of clathrin and GGA1 analyzed by fluorescence recovery after photobleaching. (A-C) MDCK cells were transiently transfected with constructs encoding GFP-clathrin (A) or GFP-GGA1 (B and C). Fluorescence associated with the Golgi complex was photobleached with high-intensity laser light and subsequent recovery of fluorescence was monitored by scanning the whole cell at low laser power at 5-s intervals for 5 min. The arrows in C indicate that the GFP-GGA1 recovers on the same TGN structures where it was located before photobleaching. N, nucleus. Bars, 10 µm (A and B), 5 µm (C). (D) Kinetics of GFP-clathrin and GFP-GGA1 recovery after photobleaching at 37 and 20°C. MDCK cells expressing GFP-clathrin or GFP-GGA1 were photobleached and then scanned at low laser power for 5 min. The graph shows the combined results of 10 determinations per condition. QuickTime videos of the experiments shown in panes A, B, and C can be seen in Supplemental Materials (videos A, B, and C).

To assess whether membrane binding and release of GFP-clathrin and GFP-GGA1 were coupled to vesicle budding from the TGN,we examined the effect of lowering the temperature to 20°C, amanipulation that blocks protein export from the TGN to variouscompartments (Griffiths et al., 1985; Xu and Shields, 1993; Wackeret al., 1997), including those of the endosomal-lysosomal system(Nishimura et al., 1990). We observed that budding of clathrin-and GGA1-containing intermediates completely ceased at this temperature(our unpublished data). Strikingly, the majority of GGA1 and clathrinfluorescence on the TGN still recovered at 20°C, albeit more slowly(Figure 9D). These results indicate that GGA1 and clathrin continueto undergo cycling on and off the TGN membrane even when vesiclebudding from the TGN is inhibited. Thus, the association and dissociationof these TGN coat proteins with membranes is not obligatorilycoupled to vesicle formation andbudding.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The results presented herein demonstrate that clathrin, GGA1, and AP-1 are associated with a population of vesicular-tubularcarriers budding from the TGN. These carriers look larger andmore pleiomorphic than conventional CCVs. After detaching fromthe TGN, the carriers move along microtubules for distances ofup to ~10 µm toward the peripheral cytoplasm. The signal of thefluorescently labeled coat proteins associated with the carriersdisappears at different times after reaching the cell periphery,probably due to uncoating. Some coated carriers, however, persistand can be seen engaging in fusion or kiss-and-run interactionswith peripheral endosomes before they lose their coat. Thus, itis likely that a function of these coated carriers is to movecargo between the TGN and peripheralendosomes.

A cargo molecule transported by these intermediates is the CD-MPR, which interacts via acidic-cluster-dileucine signals withthe VHS domain of the GGAs (Puertollano et al., 2001a; Takatsuet al., 2001; Doray et al., 2002a). Indeed, we observed that theCD-MPR leaves the TGN on vesicular-tubular structures decoratedwith GGA1. Other transmembrane proteins such as the CI-MPR (Puertollanoet al., 2001a; Takatsu et al., 2001; Zhu et al., 2001), sortilin(Nielsen et al., 2001), the low-density lipoprotein-related protein3 (Takatsu et al., 2001), and $beta$ -secretase (He et al., 2002), alsohave acidic-cluster-dileucine signals that interact with the GGAsand might therefore be exported from the TGN on the same carriers.In contrast, recycling transferrin receptors and the VSV-G proteintraffic in distinct sets of tubules and vesicles devoid ofGGA1.

The presence of both clathrin and GGA1 on the same carriers adds to the evidence that the GGAs function in association withclathrin (Puertollano et al., 2001b; Costaguta et al., 2001; Mullinsand Bonifacino, 2001). The occurrence of AP-1 on these TGN-derivedcarriers, however, is intriguing because the exact role of AP-1in sorting is currently a matter of debate. Our observations withGFP- $gamma$ 1-adaptin agree with those of Huang et al. (2001) obtainedusing YFP-µ1 to label the AP-1 complex. These authors reportedthat most YFP-µ1A-labeled vesicles also move from the TGN to theperiphery of the cells. This sense of transport contrasts withthe proposed role of AP-1 in recycling MPRs from endosomes tothe TGN, inferred from the accumulation of MPRs in peripheralendosomes of µ1A-deficient fibroblasts (Meyer et al., 2000). Apossible explanation for these seemingly contradictory observationscould be that AP-1 actually mediates removal of cargo from theintermediates as they move toward the cell periphery or upon theirmerge with peripheral endosomes. AP-1 has in fact been shown tofunction in the removal of membrane proteins from immature secretorygranules after their budding from the TGN (Klumperman et al.,1998). This would be analogous to the behavior of COPI, whichis present on vesicular tubular clusters (VTCs) moving from endoplasmicreticulum (ER) exit sites to the Golgi complex (Presley et al.,1997), even though it plays a role in protein recycling from theGolgi complex to the ER (Letourneur et al., 1994). Another possibilityis that AP-1 plays a role in sorting at the TGN, as previouslyassumed. Recent work suggests that the GGAs and AP-1 do cooperateto package MPRs into TGN-derived intermediates (Doray et al.,2002b).

The TGN-derived coated intermediates described herein seem to belong to a growing family of large intracellular transportcarriers, including VTCs, that mediate transport from the ER tothe Golgi complex (Aridor et al., 1995; Presley et al., 1997)and PGCs involved in transport of VSV-G protein from the TGN tothe plasma membrane (Hirschberg et al., 1998; Polishchuk et al.,2000). The large carriers described herein are the first onesshown to contain associated clathrin and GGA1. The decorationof tubules carrying the CD-MPR with GGA1 seem to occur in discontinuousmanner, as if defining specific domains on the tubules. The CD-MPRwas often more concentrated in the tubule domains containing associatedGGA1, suggesting that the segregation of CD-MPR from other cargomolecules may persist after budding from theTGN.

The vesicular-tubular carriers containing CD-MPR and even the individual foci labeled for clathrin, GGA1, and AP-1 were apparentlylarger than plasma membrane-coated pits and conventional CCVs.This difference could be easily appreciated in microscopic fieldswhere both types of clathrin-coated structures were visible (Figure3D). Although the intensity of the fluorescence signal can impingeupon estimations of size by optical microscopy, in the case ofclathrin it is reasonable to assume that the probability of GFP-labeledclathrin to be incorporated into clathrin lattices is the samein different parts of the cell. Thus, brighter clathrin-coatedstructures are also larger. Corroboration of the larger size ofthe TGN-derived intermediates was obtained by comparison withfluorescent beads of known size and similar brightness (Figure4). The larger size of the TGN-intermediates was not due to "streaking"because the speed of scanning (typically 20-30 µm/s) was muchhigher than the speed of the intermediates (~1 µm/s).

The fine structure of the TGN-derived carriers could not be resolved by fluorescence microscopy because of limits on the resolutionby this technique (~200 nm under the conditions of our experiments;Inoue, 1989). We envision that they consist of tubular or irregularlyshaped membrane-bound organelles (akin to VTCs [Aridor et al.,1995] or PGCs [Polishchuk et al., 2000]) with 60- to 130-nm coatedbuds that define specific domains within these organelles. Theapparently larger size of the coated foci relative to CCVs couldbe due to the presence of several 60- to 130-nm coated buds onthe carriers. It is also possible that the larger foci representclusters of CCVs that are somehow tetheredtogether.

An important property of the TGN-associated coats studied herein is that they are constantly cycling between membranes andthe cytosol. Even when vesicle budding from the TGN is inhibitedby incubation at 20°C, the coats continue to exchange. Therefore,dissociation of the coats does not require formation of vesicularintermediates. In this regard, the clathrin GGA- and AP-1-containingTGN coats behave like plasma membrane clathrin coats (Wu et al.,2001) and COPI (Presley et al., 2002), which also cycle on andoff membranes when vesicle budding is inhibited. We were unableto examine the dynamics of coats on the TGN-derived intermediatesthemselves because of their mobility. In any event, whether dynamicallyor statically, the intermediates do retain their coats until theyreach the periphery. The coats could thus be directly responsiblefor the recruitment of motor molecules that effect tracking alongmicrotubules. The kinesin superfamily protein KIF13A, for example,is a plus-end microtubule motor that interacts with the $beta$ 1-adaptinsubunit of AP-1 (Nakagawa et al., 2000). The coats could alsobind tethering proteins that allow interactions or fusion of theintermediates with endosomes. For instance, rabaptin-5 is an effectorof the early endosomal rab4 and rab5 GTP-binding proteins (Stenmarket al., 1995; Vitale et al., 1998) that also interacts with the $gamma$ 1-adaptin subunit of AP-1 (Shiba et al., 2002). The persistenceof the coats on the intermediates may thus enable their involvementin organelle targeting events, in addition to their roles in vesicleformation and cargoselection.

Of course, our observations do not rule out the existence of small CCVs that could mediate short-range transfer of cargo tothe larger intermediates or to endosomes located in the vicinityof the TGN. In fact, the endosomal recycling compartment (Yamashiroet al., 1984) and late endosomes (Rabinowitz et al., 1992) aremostly concentrated in the juxtanuclear area of the cell. It wouldbe virtually impossible to observe direct transfer of materialsfrom the TGN to these compartments. Small CCVs could also pinchoff from the large intermediates as they move toward the peripheralcytoplasm. Finally, small CCVs could be too weakly labeled ortransient for detection. Nevertheless, our findings do revealthe existence of a previously unrecognized type of intermediatecontaining associated clathrin coats, which could be involvedin long-range delivery of biosynthetic cargo to peripheral cellularlocations.

	ACKNOWLEDGMENTS

We thank Jennifer Lippincott-Schwartz for helpful discussions and Margaret S. Robinson for kind gifts ofreagents.

	FOOTNOTES

Online version of this article contains video material for some figures. Online version available at www.molbiolcell.org.

^§ Corresponding author. E-mail address: juan{at}helix.nih.gov.

Article published online ahead of print. Mol. Biol. Cell 10.1091/mbc.02-07-0109. Article and publication date are at www.molbiolcell.org/cgi/doi/10.1091/mbc.02-07-0109.

REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Aridor, M., Bannykh, S.I., Rowe, T., and Balch, W.E. (1995). Sequential coupling between COPII and COPI vesicle coats in endoplasmic reticulum to Golgi transport. J. Cell Biol. 131, 875-893[Abstract/Free Full Text].
Boman, A.L. (2001). GGA proteins: new players in the sorting game. J. Cell Sci. 114, 3413-3418[Abstract/Free Full Text].
Brodsky, F.M., Chen, C.Y., Knuehl, C., Towler, M.C., and Wakeham, D.E. (2001). Biological basket weaving: formation and function of clathrin-coated vesicles. Annu. Rev. Cell Dev. Biol. 17, 517-568[CrossRef][Medline].
Costaguta, G., Stefan, C.J., Bensen, E.S., Emr, S.D., and Payne, G.S. (2001). Yeast GGA coat proteins function with clathrin in Golgi to endosome transport. Mol. Biol. Cell 12, 1885-96[Abstract/Free Full Text].
Damer, C.K., and O'Halloran, T.J. (2000). Spatially regulated recruitment of clathrin to the plasma membrane during capping and cell translocation. Mol. Biol. Cell 11, 2151-2159[Abstract/Free Full Text].
Dell'Angelica, E.C., Puertollano, R., Mullins, C., Aguilar, R.C., Vargas, J.D., Hartnell, L.M., and Bonifacino, J.S. (2000). GGAs. A family of ADP ribosylation factor-binding proteins related to adaptors and associated with the Golgi complex. J. Cell Biol. 149, 81-94[Abstract/Free Full Text].
Doray, B., Bruns, K., Ghosh, P., and Kornfeld, S. (2002a). Interaction of the cation-dependent mannose 6-phosphate receptor with GGA proteins. J. Biol. Chem. 277, 18477-82[Abstract/Free Full Text].
Doray, B., Ghosh, P., Griffith, J., Geuze, H.J., and Kornfeld, S. (2002b). Cooperation of GGAs and AP-1 in packaging man-6-p receptors at the trans-Golgi network. Science 297, 1700-1703[Abstract/Free Full Text].
Gaidarov, I., Santini, F., Warren, R.A., and Keen, J.H. (1999). Spatial control of coated-pit dynamics in living cells. Nat. Cell Biol. 1, 1-7[CrossRef][Medline].
Griffiths, G., Pfeiffer, S., Simons, K., and Matlin, K. (1985). Exit of newly synthesized membrane proteins from the trans cisternae of the Golgi complex to the plasma membrane. J. Cell Biol. 101, 949-964[Abstract/Free Full Text].
He, X., Chang, W.P., Koelsch, G., and Tang, J. (2002). Memapsin 2 ( $beta$ -secretase) cytosolic domain binds to the VHS domains of GGA1 and GGA2: implications on the endocytosis mechanism of memapsin 2. FEBS Lett. 524, 183-7[Medline].
Hirschberg, K., Miller, C.M., Ellenberg, J., Presley, J.F., Siggia, E.D., Phair, R.D., and Lippincott-Schwartz, J. (1998). Kinetic analysis of secretory protein traffic and characterization of Golgi to plasma membrane transport intermediates in living cells. J. Cell Biol. 143, 1485-1503[Abstract/Free Full Text].
Hirst, J., Lindsay, M.R., and Robinson, M.S. (2001). GGAs. Roles of the different domains and comparison with AP-1 and clathrin. Mol. Biol. Cell 12, 3573-3588[Abstract/Free Full Text].
Huang, F., Nesterov, A., Carter, R.E., and Sorkin, A. (2001). Trafficking of yellow-fluorescent-protein-tagged µ1 subunit of clathrin adaptor AP-1 complex in living cells. Traffic 2, 345-357[CrossRef][Medline].
Inoue, S. (1989). Imaging of unresolved objects, superresolution, and precision of distance measurement with video microscopy. Methods Cell Biol. 30, 85-112[Medline].
Jacobson, K., Derzko, Z., Wu, E.S., Hou, Y., and Poste, G. (1976). Measurement of the lateral mobility of cell surface components in single, living cells by fluorescence recovery after photobleaching. J. Supramol. Struct. 5, 428.
Kirchhausen, T. (2000). Clathrin. Annu. Rev. Biochem. 69, 699-727[CrossRef][Medline].
Klumperman, J., Kuliawat, R., Griffith, J.M., Geuze, H.J., and Arvan, P. (1998). Mannose 6-phosphate receptors are sorted from immature secretory granules via adaptor protein AP-1, clathrin, and syntaxin 6-positive vesicles. J. Cell Biol. 141, 359-371[Abstract/Free Full Text].
Letourneur, F., Gaynor, E.C., Hennecke, S., Demolliere, C., Duden, R., Emr, S.D., Riezman, H., and Cosson, P. (1994). Coatomer is essential for retrieval of dilysine-tagged proteins to the endoplasmic reticulum. Cell 79, 1199-1207[CrossRef][Medline].
Meyer, C., Zizioli, D., Lausmann, S., Eskelinen, E.L., Hamann, J., Saftig, P., von Figura, K., and Schu, P. (2000). µ1a-Adaptin-deficient mice: lethality, loss of AP-1 binding and rerouting of mannose 6-phosphate receptors. EMBO J. 19, 2193-2203[CrossRef][Medline].
Mullins, C., and Bonifacino, J.S. (2001). Structural requirements for function of yeast GGAs in vacuolar protein sorting, $alpha$ -factor maturation, and interactions with clathrin. Mol. Cell. Biol. 21, 7981-7994[Abstract/Free Full Text].
Nakagawa, T., Setou, M., Seog, D., Ogasawara, K., Dohmae, N., Takio, K., and Hirokawa, N. (2000). A novel motor, kif13a, transports mannose-6-phosphate receptor to plasma membrane through direct interaction with AP-1 complex. Cell 103, 569-581[CrossRef][Medline].
Nielsen, M.S., Madsen, P., Christensen, E.I., Nykjaer, A., Gliemann, J., Kasper, D., Pohlmann, R., and Petersen, C.M. (2001). The sortilin cytoplasmic tail conveys Golgi-endosome transport and binds the VHS domain of the GGA2 sorting protein. EMBO J. 20, 2180-2190[CrossRef][Medline].
Nishimura, Y., Kawabata, T., Yano, S., and Kato, K. (1990). Inhibition of intracellular sorting and processing of lysosomal cathepsins h and l at reduced temperature in primary cultures of rat hepatocytes. Arch. Biochem. Biophys. 283, 458-463[CrossRef][Medline].
Peters, P.J. (1998). Cryo-immunogold electron microscopy. In: Current Protocols in Cell Biology, ed. J.S. Bonifacino, M. Dasso, J.B. Harford, J. Lippincott-Schwartz, and K. Yamada, New York: John Wiley & Sons, 4.7.1-4.7.12.
Polishchuk, R.S., Polishchuk, E.V., Marra, P., Alberti, S., Buccione, R., Luini, A., and Mironov, A.A. (2000). Correlative light-electron microscopy reveals the tubular-saccular ultrastructure of carriers operating between Golgi apparatus and plasma membrane. J. Cell Biol. 148, 45-58[Abstract/Free Full Text].
Porcelli, S., Morita, C.T., and Brenner, M.B. (1992). Cd1b restricts the response of human CD4-8-t lymphocytes to a microbial antigen. Nature 360, 593-597[CrossRef][Medline].
Presley, J.F., Cole, N.B., Schroer, T.A., Hirschberg, K., Zaal, K.J., and Lippincott-Schwartz, J. (1997). ER-to-Golgi transport visualized in living cells. Nature 389, 81-85[CrossRef][Medline].
Presley, J.F., Ward, T.H., Pfeiffer, A., Siggia, E.D., Phair, R.D., and Lippincott-Schwartz, J. (2002). Dissection of copi and arf1 dynamics in vivo and role in Golgi membrane transport. Nature 417, 187-193[CrossRef][Medline].
Puertollano, R., Aguilar, R.C., Gorshkova, I., Crouch, R.J., and Bonifacino, J.S. (2001a). Sorting of mannose 6-phosphate receptors mediated by the GGAs. Science 292, 1712-1716[Abstract/Free Full Text].
Puertollano, R., Randazzo, P., Hartnell, L.M., Presley, J., and Bonifacino, J.S. (2001b). The GGAs promote ARF-dependent recruitment of clathrin to the TGN. Cell 105, 93-102[CrossRef][Medline].
Rabinowitz, S., Horstmann, H., Gordon, S., and Griffiths, G. (1992). Immunocytochemical characterization of the endocytic and phagolysosomal compartments in peritoneal macrophages. J. Cell Biol. 116, 95-112[Abstract/Free Full Text].
Robinson, M.S., and Bonifacino, J.S. (2001). Adaptor-related proteins. Curr. Opin. Cell Biol. 13, 444-453[CrossRef][Medline].
Shiba, Y., Takatsu, H., Shin, H.W., and Nakayama, K. (2002). $gamma$ -Adaptin interacts directly with rabaptin-5 through its ear domain. J. Biochem. 131, 327-336[Abstract/Free Full Text].
Stenmark, H., Vitale, G., Ullrich, O., and Zerial, M. (1995). Rabaptin-5 is a direct effector of the small GTPase rab5 in endocytic membrane fusion. Cell 83, 423-432[CrossRef][Medline].
Storrie, B., and Desjardins, M. (1996). The biogenesis of lysosomes: is it a kiss and run, continuous fusion and fission process? Bioessays 18, 895-903[CrossRef][Medline].
Takatsu, H., Katoh, Y., Shiba, Y., and Nakayama, K. (2001). Golgi-localizing, $gamma$ -adaptin ear homology domain, ADP-ribosylation factor-binding (GGA) proteins interact with acidic dileucine sequences within the cytoplasmic domains of sorting receptors through their vps27p/hrs/stam (VHS) domains. J. Biol. Chem. 276, 28541-28545[Abstract/Free Full Text].
Vitale, G., Rybin, V., Christoforidis, S., Thornqvist, P., McCaffrey, M., Stenmark, H., and Zerial, M. (1998). Distinct rab-binding domains mediate the interaction of rabaptin-5 with GTP-bound rab4 and rab5. EMBO J. 17, 1941-1951[CrossRef][Medline].
Wacker, I., Kaether, C., Kromer, A., Migala, A., Almers, W., and Gerdes, H.H. (1997). Microtubule-dependent transport of secretory vesicles visualized in real time with a GFP-tagged secretory protein. J. Cell Sci. 110, 1453-63[Abstract].
Wu, X., Zhao, X., Baylor, L., Kaushal, S., Eisenberg, E., and Greene, L.E. (2001). Clathrin exchange during clathrin-mediated endocytosis. J. Cell Biol. 155, 291-300[Abstract/Free Full Text].
Xu, H., and Shields, D. (1993). Prohormone processing in the trans-Golgi network: endoproteolytic cleavage of prosomatostatin and formation of nascent secretory vesicles in permeabilized cells. J. Cell Biol. 122, 1169-1184[Abstract/Free Full Text].
Yamashiro, D.J., Tycko, B., Fluss, S.R., and Maxfield, F.R. (1984). Segregation of transferrin to a mildly acidic (ph 6.5) para-Golgi compartment in the recycling pathway. Cell 37, 789-800[CrossRef][Medline].
Zhu, Y., Doray, B., Poussu, A., Lehto, V.P., and Kornfeld, S. (2001). Binding of GGA2 to the lysosomal enzyme sorting motif of the mannose 6-phosphate receptor. Science 292, 1716-1718[Abstract/Free Full Text].

This article has been cited by other articles:

R. C. N. Melo, L. A. Spencer, A. M. Dvorak, and P. F. Weller
Mechanisms of eosinophil secretion: large vesiculotubular carriers mediate transport and release of granule-derived cytokines and other proteins
J. Leukoc. Biol., February 1, 2008; 83(2): 229 - 236.
[Abstract] [Full Text] [PDF]

G. A. Mardones, P. V. Burgos, D. A. Brooks, E. Parkinson-Lawrence, R. Mattera, and J. S. Bonifacino
The Trans-Golgi Network Accessory Protein p56 Promotes Long-Range Movement of GGA/Clathrin-containing Transport Carriers and Lysosomal Enzyme Sorting
Mol. Biol. Cell, September 1, 2007; 18(9): 3486 - 3501.
[Abstract] [Full Text] [PDF]

G. Camus, C. Segura-Morales, D. Molle, S. Lopez-Verges, C. Begon-Pescia, C. Cazevieille, P. Schu, E. Bertrand, C. Berlioz-Torrent, and E. Basyuk
The Clathrin Adaptor Complex AP-1 Binds HIV-1 and MLV Gag and Facilitates Their Budding
Mol. Biol. Cell, August 1, 2007; 18(8): 3193 - 3203.
[Abstract] [Full Text] [PDF]

S. Wasiak, R. Zunino, and H. M. McBride
Bax/Bak promote sumoylation of DRP1 and its stable association with mitochondria during apoptotic cell death
J. Cell Biol., May 7, 2007; 177(3): 439 - 450.
[Abstract] [Full Text] [PDF]

F. Zhang, Y.-I. Yim, S. Scarselletta, M. Norton, E. Eisenberg, and L. E. Greene
Clathrin Adaptor GGA1 Polymerizes Clathrin into Tubules
J. Biol. Chem., May 4, 2007; 282(18): 13282 - 13289.
[Abstract] [Full Text] [PDF]

A. Copic, T. L. Starr, and R. Schekman
Ent3p and Ent5p Exhibit Cargo-specific Functions in Trafficking Proteins between the Trans-Golgi Network and the Endosomes in Yeast
Mol. Biol. Cell, May 1, 2007; 18(5): 1803 - 1815.
[Abstract] [Full Text] [PDF]

Y. Zhao, I. Gaidarov, and J. H. Keen
Phosphoinositide 3-Kinase C2{alpha} Links Clathrin to Microtubule-dependent Movement
J. Biol. Chem., January 12, 2007; 282(2): 1249 - 1256.
[Abstract] [Full Text] [PDF]

J. C. Hou, N. Suzuki, J. E. Pessin, and R. T. Watson
A Specific Dileucine Motif Is Required for the GGA-dependent Entry of Newly Synthesized Insulin-responsive Aminopeptidase into the Insulin-responsive Compartment
J. Biol. Chem., November 3, 2006; 281(44): 33457 - 33466.
[Abstract] [Full Text] [PDF]

C. Foote and S. F. Nothwehr
The clathrin adaptor complex 1 directly binds to a sorting signal in Ste13p to reduce the rate of its trafficking to the late endosome of yeast
J. Cell Biol., May 22, 2006; 173(4): 615 - 626.
[Abstract] [Full Text] [PDF]

L. Xie, D. Boyle, D. Sanford, P. E. Scherer, J. E. Pessin, and S. Mora
Intracellular Trafficking and Secretion of Adiponectin Is Dependent on GGA-coated Vesicles
J. Biol. Chem., March 17, 2006; 281(11): 7253 - 7259.
[Abstract] [Full Text] [PDF]

E. E. Heldwein, E. Macia, J. Wang, H. L. Yin, T. Kirchhausen, and S. C. Harrison
Crystal structure of the clathrin adaptor protein 1 core
PNAS, September 28, 2004; 101(39): 14108 - 1411

				G. A. Mardones, P. V. Burgos, D. A. Brooks, E. Parkinson-Lawrence, R. Mattera, and J. S. Bonifacino The Trans-Golgi Network Accessory Protein p56 Promotes Long-Range Movement of GGA/Clathrin-containing Transport Carriers and Lysosomal Enzyme Sorting Mol. Biol. Cell, September 1, 2007; 18(9): 3486 - 3501. [Abstract] [Full Text] [PDF]

				G. Camus, C. Segura-Morales, D. Molle, S. Lopez-Verges, C. Begon-Pescia, C. Cazevieille, P. Schu, E. Bertrand, C. Berlioz-Torrent, and E. Basyuk The Clathrin Adaptor Complex AP-1 Binds HIV-1 and MLV Gag and Facilitates Their Budding Mol. Biol. Cell, August 1, 2007; 18(8): 3193 - 3203. [Abstract] [Full Text] [PDF]

				S. Wasiak, R. Zunino, and H. M. McBride Bax/Bak promote sumoylation of DRP1 and its stable association with mitochondria during apoptotic cell death J. Cell Biol., May 7, 2007; 177(3): 439 - 450. [Abstract] [Full Text] [PDF]

				F. Zhang, Y.-I. Yim, S. Scarselletta, M. Norton, E. Eisenberg, and L. E. Greene Clathrin Adaptor GGA1 Polymerizes Clathrin into Tubules J. Biol. Chem., May 4, 2007; 282(18): 13282 - 13289. [Abstract] [Full Text] [PDF]

				A. Copic, T. L. Starr, and R. Schekman Ent3p and Ent5p Exhibit Cargo-specific Functions in Trafficking Proteins between the Trans-Golgi Network and the Endosomes in Yeast Mol. Biol. Cell, May 1, 2007; 18(5): 1803 - 1815. [Abstract] [Full Text] [PDF]

				Y. Zhao, I. Gaidarov, and J. H. Keen Phosphoinositide 3-Kinase C2{alpha} Links Clathrin to Microtubule-dependent Movement J. Biol. Chem., January 12, 2007; 282(2): 1249 - 1256. [Abstract] [Full Text] [PDF]

				J. C. Hou, N. Suzuki, J. E. Pessin, and R. T. Watson A Specific Dileucine Motif Is Required for the GGA-dependent Entry of Newly Synthesized Insulin-responsive Aminopeptidase into the Insulin-responsive Compartment J. Biol. Chem., November 3, 2006; 281(44): 33457 - 33466. [Abstract] [Full Text] [PDF]

				C. Foote and S. F. Nothwehr The clathrin adaptor complex 1 directly binds to a sorting signal in Ste13p to reduce the rate of its trafficking to the late endosome of yeast J. Cell Biol., May 22, 2006; 173(4): 615 - 626. [Abstract] [Full Text] [PDF]

				L. Xie, D. Boyle, D. Sanford, P. E. Scherer, J. E. Pessin, and S. Mora Intracellular Trafficking and Secretion of Adiponectin Is Dependent on GGA-coated Vesicles J. Biol. Chem., March 17, 2006; 281(11): 7253 - 7259. [Abstract] [Full Text] [PDF]