Role of Dynactin in Endocytic Traffic: Effects of Dynamitin Overexpression and Colocalization with CLIP-170

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Vol. 10, Issue 12, 4107-4120, December 1999

Role of Dynactin in Endocytic Traffic: Effects of Dynamitin Overexpression and Colocalization with CLIP-170

Caterina Valetti,^* Dawn M. Wetzel,^§ Michael Schrader, M. Josh Hasbani,^¶ Steven R. Gill,^# Thomas E. Kreis,^* and Trina A. Schroer^**

^*Department of Cell Biology, University of Geneva, Geneva 1211, Switzerland; and Department of Biology, The Johns Hopkins University, Baltimore, Maryland 21218

Submitted June 17, 1999; Accepted September 23, 1999
Monitoring Editor: Suzanne R. Pfeffer

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The flow of material from peripheral, early endosomes to late endosomes requires microtubules and is thought to be facilitatedby the minus end-directed motor cytoplasmic dynein and its activatordynactin. The microtubule-binding protein CLIP-170 may also playa role by providing an early link to endosomes. Here, we showthat perturbation of dynactin function in vivo affects endosomedynamics and trafficking. Endosome movement, which is normallybidirectional, is completely inhibited. Receptor-mediated uptakeand recycling occur normally, but cells are less susceptible toinfection by enveloped viruses that require delivery to late endosomes,and they show reduced accumulation of lysosomally targeted probes.Dynactin colocalizes at microtubule plus ends with CLIP-170 ina way that depends on CLIP-170's putative cargo-binding domain.Overexpression studies using p150^Glued, the microtubule-binding subunit of dynactin, and mutant andwild-type forms of CLIP-170 indicate that CLIP-170 recruits dynactinto microtubule ends. These data suggest a new model for the formationof motile complexes of endosomes and microtubules early in theendocyticpathway.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The microtubule cytoskeleton provides a dynamic structural framework that underlies a wide variety of subcellular motile events.The steady-state localizations of endomembrane systems such asthe endoplasmic reticulum (ER), Golgi apparatus, endosomes, andlysosomes require both intact microtubules and the activitiesof microtubule-based motor proteins (reviewed by Goodson et al.,1997). The extension of ER tubules, the Golgi-to-ER "recycling"leg of the biosynthetic pathway, and the centrifugal movementof lysosomes are thought to require the activity of a plus end-directedmotor such as kinesin or a kinesin-related protein (reviewed byLane and Allan, 1998). Cytoplasmic dynein, the predominant cytosolicminus end-directed motor, in conjunction with its activator, dynactin(Gill et al., 1991), maintains the Golgi complex, endosomes, andlysosomes in the normal juxtanuclear position (Burkhardt et al.,1997; Harada et al., 1998). Dynein/dynactin drives membrane transportfrom the ER to the Golgi complex (Presley et al., 1997) and mayfacilitate inward flow of material within the endocytic pathway,as suggested by in vitro studies of protein transfer from earlyto late endosomes (Bomsel et al., 1990; Aniento et al., 1993).However, the contributions of dynein and dynactin to endocytictrafficking in vivo have yet to be determined, because previousdynein antibody microinjection studies (Vaisberg et al., 1993;Burkhardt et al., 1997) and evaluation of dynein knock-out mice(Harada et al., 1998) did not address endosome function in detail.An in-depth exploration of the effects of dynein/dynactin perturbationon endocytic trafficking and dynamics in living cells is clearlywarranted.

The cytoplasmic dyneins are a multiprotein family of at least three members (Criswell et al., 1996; Vaisberg et al., 1996).The most abundant isoform, dynein 1, works in conjunction witha multisubunit activator protein, dynactin. Dynactin is thoughtto serve as an adapter that mediates dynein binding to a varietyof cargo structures, including membranes, chromosomes and microtubules(reviewed by Allan, 1996; Holleran et al., 1998). It is also proposedto facilitate long-range movement by increasing dynein processivity(King and Schroer, 2000). To allow for these different functions,dynactin has two distinct structural domains (Schafer et al.,1994). Its rigid, filamentous backbone contains several proteinswhose sequences predict both covalent and noncovalent cargo attachmentmechanisms (Eckley et al., 1999), whereas its flexible projectingsidearm binds dynein and microtubules (reviewed by Holleran etal., 1998). These two domains are thought to be linked by theprotein dynamitin which, when overexpressed, causes dynactin'ssidearm to release from the backbone (Echeverri et al., 1996),thus decoupling dynein-binding and cargo-anchoring functions.This leads to a variety of defects; mitotic cells arrest in pseudoprometaphase(Echeverri et al., 1996), whereas interphase cells show alteredsteady-state distributions of the Golgi complex, endosomes, andlysosomes (Burkhardt et al., 1997). Addition of excess dynamitinto cell extracts (Wittman and Hyman, 1999) and purified dynactin(Eckley et al., 1999) also disrupts dynactin structure, suggestingthat it can also be used to impair dynein-dependent activitiesin vitro. Dynamitin is thus a powerful tool for analyzing dynactinand, by inference, dynein, function in a variety ofcontexts.

Endosomes in the cell periphery are believed to be transiently tethered to microtubules via the cytoplasmic linker proteinCLIP-170 before centripetal movement (Rickard and Kreis, 1996).CLIP-170 contributes to the binding of endosomal membranes tomicrotubules in vitro (Pierre et al., 1992). In cells, CLIP-170labels the growing ends of microtubules (Perez et al., 1999),an appropriate site for its proposed function. Microtubule bindingis regulated by phosphorylation (Rickard and Kreis, 1991), providinga means for release of CLIP-170 (and associated cargo) from microtubulesunder circumstances in which a static interaction is no longerneeded. This might occur once motors have been recruited to theendosome-microtubulecomplex.

In the present study, we examine the contribution of the dynein/dynactin motor to endocytic motility and trafficking and exploreits links to CLIP-170. Late endosomes located near the centerof the cell move bidirectionally over long distances. In cellsthat overexpress dynamitin, this movement, and that of other organelles,is completely inhibited. Membranes of the endocytic pathway accumulatein the cell periphery, as seen previously. Although early andlate endosomes are now in close proximity, forward traffic throughthe pathway is slowed. The highly conserved dynamitin N terminusis found to be sufficient to inhibit dynactin activity in vivo.In immunolocalization studies, dynactin colocalizes with CLIP-170at microtubule plus ends, an association that depends on the CLIP-170C-terminal cargo-binding domain. This suggests that CLIP-170 bindsto microtubules first and then recruits dynactin, providing aconcerted mechanism for loading endosomes onto microtubules andconverting them to a motilepool.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Cell Lines

Vero (CCL81; American Type Culture Collection, Manassas, VA) and HeLa (CCL2; American Type Culture Collection) were grownin minimum essential medium plus 1% glutamine and 5 or 10% FCS.Cos7 cells were grown in Dulbecco's modified Eagle's medium and10%FCS.

Antibodies

Rabbit Abs were CLIP-170 (Ab 55; Pierre et al., 1992), influenza hemagglutinin (HA; Daro et al., 1996), MPR300 (a gift fromO. Rosorius, University of Geneva), early endosomal antigen 1(EEA1) (Simonsen et al., 1998), vesicular stomatitis virus glycoprotein(VSV-G; Griffiths et al., 1985), pAb p150^Glued (Vaughan et al., 1999), and pAb dynamitin antiserum to dynamitingel purified from bovinedynactin.

Mouse mAbs were anti-HA-epitope (Daro et al., 1996), lysobisphosphatidic acid (LBPA mAb 6C4 (Kobayashi et al., 1998), anti-transferrin(Tfn)-R mAb OKT9 (Sutherland et al., 1981), anti-giantin (Linstedtand Hauri, 1993), mAb P5D4 against the VSV-G cytoplasmic tail(Kreis, 1986), anti-galactosyltransferase (Kawano et al., 1994),anti-myc epitope mAb 9E10 (Evan et al., 1985), CD63 mAb 1B5 (agift from M. Marsh, University College, London, United Kingdom),and CLIP-170 mAbs 2D6 and 4D3 (Rickard and Kreis, 1991; Pierreet al., 1992). The anti-dynamitin mAb 50A (chicken specific) andanti-p150^Glued mAb 150B were isolated in the same monoclonal screen that yieldedmAbs 45A and 62B (Schafer et al., 1994). Anti- $beta$ -galactosidase( $beta$ -gal) was from Promega (Madison,WI).

Dynamitin Cloning

A $lambda$ gtll chick embryo library (B. Vennstrom, European Molecular Biology Laboratory, Heidelberg, Germany) was screened usingmAb 50A. cDNAs from immunopositive clones were isolated, digestedwith EcoRI, and ligated into the EcoRI site of pBluescript KSII+ (Stratagene, La Jolla, CA) for later manipulations. NestedExoIII deletions of the longest dynamitin cDNA (1.5 kb) were sequencedusing Sequenase (Amersham Life Science, Arlington Heights, IL),and the sequence from both strands was assembled using the MacDNasisDNA analysis program (Hitachi Software Engineering, San Bruno,CA).

Expression Constructs

The dynamitin cDNA insert was subcloned into two cytomegalovirus (CMV)-based expression vectors: pGW1-CMV (Quintyne et al.,1999) and pCB6 containing an upstream HA tag (Balda et al., 1996).To facilitate subcloning, the first 108 bp of the dynamitin cDNAwas amplified by PCR using an AlfII site introduced at the dynamitininitiator codon and a unique, downstream SacI site. The remainderof dynamitin was cloned from the SacI and XbaI sites, and thetwo fragments were religated into pCB6-HA. The dynamitin N terminus(amino acids 1-87) cDNA was made by reverse transcriptase-PCRfrom the original $lambda$ gt11 clone and subcloned in pTA (Invitrogen,Carlsbad, CA). The insert was verified by sequencing and clonedinto pGW1-CMV. A $lambda$ gt10 insert encoding full-length chicken p150was cloned as described (Quintyne et al., 1999). Plasmid pSG5-myc-CLIP-170wild type (wt) contained the EcoRI insert from pGEM-myc-CLIP (Pierreet al., 1994) subcloned into pSG5; pSG5-myc-CLIP $Delta$ 1240 was generatedby truncating pSG5-myc-CLIP-170 wt using XhoI and BamHI followedby blunting and religation (both were gifts from J. Rickard, Universityof Geneva). pSG5-Sar1p contained Sar1p cDNA (from B. Balch, ScrippsInstitute, La Jolla, CA; Aridor et al., 1995) subcloned into pSG5(a gift from M. Gomez, University of Geneva). CMV-based vectorsencoding humanized green fluorescent protein (GFP) and a red-shiftedGFP (pCGFP2) were gifts from W.J. Nelson (Stanford University,Stanford, CA) and D. Shima and G. Warren (Imperial Cancer ResearchFund, London, United Kingdom),respectively.

Transfection and Microinjection of Plasmids

HeLa and Vero cells, plated on 10-mm² coverslips 24 h before transfection, were transfected (CaPO₄) with Qiagen (Santa Clarita,CA)-purified plasmid DNAs (15 µg/dish) and analyzed 24-36 h later.Cos7 cells plated on 31-mm round or 22-mm² square coverslips 24-48 h before transfection were transfected(LipofectAMINE; Life Technologies, Gaithersburg, MD) with CsCl-purifiedplasmid DNAs (dynamitin, 4 µg/ml; dynamitin N terminus; GFP, 1µg/ml) and analyzed 20-30 h later. DNA was microinjected intoVero cell nuclei using an automated microinjection system (AIS;Zeiss, Thornwood, NY) as described (Scales et al., 1997). Microinjectedcells were incubated at 37°C for 3-4 h before virusinfection.

Virus Infection

Vero cells (36-40 h after transfection or 3-4 h after microinjection) were infected with temperature-sensitive Orsay 45 (ts-O45)VSV for 1 h at 17-20°C, 1.5 or 2 h at 20°C, or 1 or 2 h at 37°Cand then incubated at the nonpermissive temperature (39.5°C) for3 h as described (Kreis, 1986).

Immunofluorescence

Cells were fixed in $-$ 20°C methanol or 3% paraformaldehyde in PBS and then permeabilized with 0.05% saponin, or with 3.7% formaldehydein PBS and then permeabilized with 0.1% Triton-X-100, before beingstained with antibodies and observed on Zeiss Axiovert 35 or TV135microscopes. Images were recorded as described (Pepperkok et al.,1993).

Assay for Dynactin Integrity

Dynactin integrity was assayed as previously described (Echeverri et al., 1996). Briefly, cells on three 10-cm dishes weretransfected and grown for 30 h. Transfection efficiency was monitoredby including, in each dish, a coverslip that was fixed and stainedat harvest. The remaining cells were harvested using PBS-EDTA,washed, and solubilized in an equal volume of lysis buffer (Echeverriet al., 1996). Cell lysates were clarified by centrifugation,the supernatants were centrifuged into sucrose gradients, andgradient fractions were analyzed onimmunoblots.

Labeling with Endocytic Tracers

$alpha$ ₂-Macroglobulin ( $alpha$ ₂-M; Calbiochem, La Jolla, CA) or Tfn (Sigma, St. Louis, MO) was conjugated with Cy3 or FITC/Fluor-X (Amersham)according to the manufacturer's protocol. Dye-protein conjugateswere isolated on desalting columns; dye:protein ratios of 1:1.25were obtained. Cells were incubated with Cy3-Tfn or $alpha$ ₂-M for analysisof probe uptake, accumulation, ormotility.

Cos7 Cells. Before Tfn uptake, cells were serum starved ( $>=$ 1 h at 37°C). Cells labeled with both C₅-dimethyl BODIPY (DMB)-ceramide (MolecularProbes, Eugene, OR) and Tfn were serum starved before Golgi labeling.Cells were then incubated at 37°C with Cy3-Tfn (10-15 µg/ml) for10 min or Cy3- $alpha$ ₂-M (60-200 µg/ml) for 20 min. For uptake and accumulationstudies, cells were rinsed for 2 min at 37°C and then fixed (Tfnand $alpha$ ₂-M) or chased for 90 min before fixation ( $alpha$ ₂-M only). Foreach cell, labeling intensity (bright, dim, or no label) was scored,and the predominant location of fluorescence (e.g., central, random,or peripheral) was determined by eye. For motility studies, coverslipswere rinsed by dipping 2 × 50 ml of 37°C HEPES-buffered mediumplus 0.2% BSA beforeimaging.

HeLa Cells. Cells were serum starved for 1 h at 37°C in medium containing glutamine and 0.5% BSA, then labeled with 25 µg/ml FITC-Tfnfor 30 min to 1 h. The coverslips were washed for 1 min and thenfixed in 3% paraformaldehyde followed by $-$ 20°C methanol. Cellswere labeled with Cy3- $alpha$ ₂M for 10-30 min, washed, and then chasedfor 5 min or 1 h at 37°C.

Kinetic Analysis of FITC-Tfn Cycling

To examine uptake, cells grown on coverslips were serum starved as above and then pulse labeled for 2.5, 5, 10, 20, or 60min with 50 µg/ml FITC-Tfn. To examine recycling, coverslips werepulse labeled with 50 µg/ml FITC-Tfn for 1 h and then washed for30 s and chased for 5, 10, 20, or 60 min in 2 ml in medium containing10% FCS. At the end of each labeling and chase interval, coverslipswere washed for 30 s and then fixed in 3% paraformaldehyde followedby $-$ 20°C methanol. Cells overexpressing dynamitin were identifiedusing Abs the HA epitope tag. To quantify Tfn fluorescence, thecells were imaged using a charge-coupled device camera with afixed data collection time. Images were saved as nonByte images.The periphery of each cell analyzed was defined manually. Datawere analyzed using IPLab software (Scanalytics, Fairfax, VA)as described (Scales et al., 1997).

Live Cell Motility Assay

For video-enhanced fluorescence microscopy (VEFM), cells were grown on 31-mm round glass coverslips. For video-enhanced differentialinterference contrast (VEDIC) microscopy, cells were grown on22-mm² glass coverslips. The cells were transfected, stained with C₅-DMB-ceramide(Pagano et al., 1991), and then loaded with endocytic tracersas above. To verify that Golgi morphology was a reliable indicatorof dynamitin overexpression, cells were stained for Golgi (giantinmAb) and dynamitin (pAb dynamitin). Of 3000 cells evaluated inthree separate experiments, <6% in the controls had disruptedGolgi apparatus compared with 96% of dynamitin overexpressers.Cells overexpressing GFP were identified by directobservation.

Cells in HEPES-buffered medium (without phenol red) plus 5% FCS were observed by VEDIC microscopy at room temperature. ForVEFM, coverslips were mounted in 37°C medium in a heating stage(Biophysica Technologies, Towson, MD) on a Zeiss Axiovert 35TVmicroscope and kept covered to minimize evaporation. Temperaturewas monitored continuously and remained between 32 and 37°C. Cellscould be kept on the microscope for longer than 2 h; particlemovements continued, and the cells did not develop vacuoles orretractionfibers.

Cells exhibiting bright fluorescence were imaged through a 2× optovar using a silicon-intensified target camera (C-2500; Hamamatsu,Hamamatsu City, Japan) mounted on an intensifier (VideoScope International,Washington DC) to provide additional intensification and magnification.Data was recorded on a frame-addressable Hi8 videocassette recorder(EVO-9650; Sony, Tokyo, Japan). Video fields could be viewed continuouslyfor several minutes with little reduction in particlemotility.

Video Analysis

Particle tracks were traced from the video monitor onto transparency sheets. Run lengths and start and stop frames for eachmovement were used to calculate velocities. A movement was definedas a saltation at a single velocity of $>=$ 0.3 µm. For particlesundergoing multiple movements, each individual saltation was scoredseparately. The frustule spacing of the diatom Pleurosigma angulatumprovided a magnification standard. Multiple coverslips were labeledwith each marker, and 5-10 cells were viewed per coverslip perexperiment. For analysis, cells were selected that had similarsizes and shapes. Multiple experiments wereperformed.

Measurement of Endosome pH

Endosomal pH was measured using an FITC pH ratio imaging technique (Kim et al., 1996). Cells overexpressing dynamitin wereidentified on the basis of Golgi morphology (Texas Red ceramidestaining; Molecular Probes), loaded with FITC- $alpha$ ₂-M (0.4 mg/ml)for 20 min at 37°C, then mounted in the heating stage of the microscope.Excitation at 440 and 490 nm was provided by a xenon lamp andtwo monochromators (Deltascan 4000; Photon Technology International,South Brunswick, NJ). The fluorescence intensity (emission cutoff,535 ± 20 nm) of random fields was imaged with a slow scan charge-coupleddevice camera (VME200A; Photometrics, Tucson, AZ) and the 490:440ratio was calculated (Ratiotool software; Inovision, Durham, NC).At the end of each experiment, a calibration curve of fluorescenceintensity versus pH was generated in situ (Kim et al., 1996) andused to estimate the pH of individual fluorescentparticles.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

The Dynamitin N Terminus Is Sufficient to Perturb Dynactin Function

To identify conserved and potentially functionally important domains of dynamitin, we cloned and sequenced the chicken homologue.Its primary sequence predicts a protein of 45,052 M_r and a pIof 4.75 with 80% overall identity to the human protein. Comparisonwith available dynamitin sequences (human, bovine, budding yeastJnm1p, C. elegans putative 37.2-kDa protein, and mouse and Drosophilamelanogaster expressed sequence tags [ESTs]) reveals several predictedcoiled coils and a possible DNA-binding motif (Echeverri et al.,1996) that are conserved between species. Dynamitins show thehighest similarity (97% human vs. chicken and 65% human vs. fly)in the amino-terminal region (Figure 1) and complete conservationof the first 35 amino acids among vertebrates, suggesting thatthis part of the protein might also be important for function.

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Figure 1. Homology plots of chicken versus human and fly dynamitin sequences. Plots were drawn to highlight the regions of highest homology between species. Chicken, GenBank accession number AF200744; human, accession number AAC50423; fly, for AA 1-184, EST 81725; for AA 297-380, EST AA802366, for AA 1-34 and 137-380, genomic clone AC007471.

Overexpression of dynamitin in cultured cells causes the dynein-binding p150^Glued sidearm to be released from the cargo-binding, actin-relatedprotein 1 (Arp1) filament (reviewed by Allan, 1996; Schroer, 1996;Vallee and Sheetz, 1996; Holleran et al., 1998). The ensuing perturbationof dynein targeting causes mitotic defects (Echeverri et al.,1996) and altered endomembrane organization in interphase cells(Burkhardt et al., 1997). We found membranes of the cis-Golginetwork/Golgi apparatus (ER-Golgi intermediate compartment-positive/GFP-N-acetylglucosamine transferase; our unpublished results) and trans-Golginetwork (TGN; mannose-6-phosphate receptor-positive; Figure 2h)to be disrupted and dispersed upon overexpression of chicken dynamitin.The distributions of endocytic organelles were also altered (Figure2), although not all endosome subcompartments were affected inthe same way. Late endosomes (lysobisphosphatidic acid-positive;Figure 2d) and lysosomes (CD63-positive; our unpublished results)accumulated in clusters at the cell periphery. Early and recyclingendosomes (positive for the early endosome antigen EEA1; Figure2b; Tfn-R; Figure 2f) also redistributed away from the centerof the cell. Some Tfn-R-labeled structures were seen at the periphery,and some appeared to be clustered, but this redistribution wasnot as dramatic as for late endosomes and lysosomes. In contrast,endosomes stained for EEA1 were dispersed evenly throughout thecell, which suggests a difference in the behaviors of early andrecycling endosomes. No effect was detected on ER structure (calnexin-positive;our unpublished results).

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Figure 2. Effect of HA-dynamitin overexpression on the steady-state localization of early endosomes, late endosomes, and TGN. Cells were double labeled for dynamitin (HA; a, c, e, and g), early endosomes (EEA1, b; Tfn-R, f), late endosomes (LBPA; d), and TGN (MPR, mannose-6-phosphate receptor; h). Cells overexpressing HA-dynamitin are marked with asterisks. HeLa cells in a-d were fixed with 3% paraformaldehyde, and cells in e-h were fixed with MeOH. Bar, 20 µm.

Overexpression of the highly conserved N-terminal 87 amino acids of dynamitin (Figure 1) had similar disruptive effects onendosome distribution (our unpublished results) and Golgi complexorganization (Figure 3A; 69% of cells; n = 675) to the full-lengthprotein. However, sedimentation analysis of cytosolic dynactinrevealed no effect on dynactin structure (Figure 3B), unlike thefull-length dynamitin control (Echeverri et al., 1996). Apparently,the dynamitin N terminus disrupts membrane organization withoutaltering dynactin structure.

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Figure 3. Dynamitin N terminus disrupts Golgi organization but not dynactin structure. (A) Cos7 cells transfected with the highly conserved dynamitin N terminus (AA 1-87) were stained for dynamitin (pAb dynamitin; left) and the Golgi complex (giantin; right). (B) Lysates of Cos7 cells transfected with $beta$ -gal, dynamitin N terminus, or HA-dynamitin were analyzed by velocity sedimentation (Echeverri et al., 1996

). Transfection efficiency was $>=$ 50%. Gradient fractions were immunoblotted with antibodies to p150^Glued, p62, and Arp1. Sedimentation standards are indicated.

Dynactin Disruption Inhibits Bidirectional Organelle Movement but Not Endocytosis and Recycling

Dynamitin overexpression results in an accumulation of late endosomes and lysosomes at the cell periphery (Burkhardt et al.,1997; Figure 2), whereas microtubule poisons cause these organellesto become randomly distributed. This observation led Burkhardtet al. (1997) to suggest that dynamitin overexpression selectivelyinhibits dynein-based motility but not movement driven by kinesinand other kinesin family members (the "balance of power" modelfor endosome and lysosome distribution). This hypothesis is supportedby the observation that ER structure, which depends on ongoingplus end-directed motility, is not affected. However, other studieshave shown that plus and minus end-directed movements of bidirectionalparticles are tightly coupled, so both are enhanced or inhibitedin unison (Hamm-Alvarez et al., 1993; Welte et al., 1998). Inour analysis, we observed that only some endosomal subcompartmentswere concentrated at the extreme periphery of dynamitin-overexpressingcells (Figure 2), suggesting that the balance of power model mightonly hold for a subset of endosomes. To gain a clearer understandingof the impact of dynamitin overexpression on bidirectional organellemotility, we turned to live cells in which the movements of endosomesand other subcellular particles could be imageddirectly.

Cells were observed using VEDIC and VEFM, and the movements of two classes of organelle were quantified. Cells overexpressingdynamitin were identified by their disrupted Golgi complexes usingthe vital Golgi dye C₅-DMB-ceramide (Pagano et al., 1991). Ascontrols, untransfected cells, cells overexpressing cytosolicGFP, and cells in the transfected population that were not overexpressingdynamitin wereexamined.

Using VEDIC microscopy we analyzed the movement of the conspicuous, highly motile, cytoplasmic particles present in many fibroblasts.Nile Red staining revealed these to be lipid droplets (our unpublishedresults). Under normal conditions, lipid droplets undergo long-and short-range microtubule-based movements toward and away fromthe cell center and, on occasion, parallel to the cell margin(Hamm-Alvarez et al., 1993; Bulinski et al., 1997) These behaviorsindicated that lipid droplets are capable of both plus end-directedand minus end-directed movement. High levels of motility wereseen in untransfected cells and in the two transfection controls(Table 1). In contrast, lipid droplets in cells overexpressingdynamitin showed almost no movement. All motility was inhibited,suggesting that more than one motor had been affected. The lipiddroplets did not accumulate at the cell periphery (our unpublishedresults) suggesting that, for these organelles, the balance ofpower model did not hold.

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Table 1. Organelle motility

We then investigated the movement of endosomes, which are known to rely on microtubules and dynein for their steady-statedistribution in vivo (Matteoni and Kreis, 1987; Burkhardt et al.,1997). Microtubules and dynein also contribute to endocytic traffickingand fusion in vivo and in vitro, suggesting that endosome motilitymight contribute to function as well as steady-state localization(Gruenberg et al., 1989; Bomsel et al., 1990; Aniento et al.,1993). We visualized early endosomes using Tfn conjugated withthe brilliantly fluorescent, photo-stable dye Cy3. Cells werebriefly loaded with the probe and immediately viewed by VEFM.In control Cos7 and HeLa cells, Tfn first appeared in irregularlyshaped structures (0.2-2 µm diameter) in the periphery ("sortingendosomes") and near the nucleus ("recycling endosomes"). Thisdistribution was similar to that of endosomes stained for Tfn-R(e.g., Figure 2f; Gruenberg and Maxfield, 1995) or endosomes stainedfor the peripherally associated early endosomal protein EEA1 (Muet al., 1995; Figure 2b). A qualitative assessment of Tfn uptakein dynamitin overexpressers indicated that most cells had internalizedthe probe (Figure 4B). However, Tfn was delivered to structuresthat were more peripherally distributed than in controls (Figures4A, right panel, and 5D). Although these organelles showed someoverlap with late endosomes, the two compartments did not completelycolocalize (Figure 4A). Quantitative analysis of the Tfn cyclein individual cells (Figure 4C) revealed that dynamitin overexpresserstook up and recycled Tfn as efficiently as controls, despite thealtered localization of the recycling compartment. This findingcorroborates recent work in Madin-Darby canine kidney cells showingthat receptor recycling can occur from early endosomes in theperiphery (Sheff et al., 1999).

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Figure 4. Tfn trafficking in control and dynamitin-overexpressing cells. (A) HeLa cells were labeled with FITC-Tfn for 1 h and then fixed (paraformaldehyde followed by MeOH) and stained for the late endosome marker LBPA (left). Inset, boxed area at 2× magnification. Cells overexpressing HA-dynamitin are marked with asterisks. (B) Qualitative analysis of uptake. Transfected Cos7 cells were labeled with Cy3-Tfn for 20 min and then fixed. Dynamitin overexpressers (i.e., cells with disrupted Golgi complexes) and control cells were scored as bright or dim (n = 180 cells total). (C) Quantitative analysis of Tfn uptake and recycling. HeLa cells were fixed after increasing times of labeling (0-60 min) or after 1 h of labeling and 0-60 min of chase. The fluorescence intensities of $>=$ 15 control (solid lines) or dynamitin-overexpressing (dotted lines) cells were measured, and mean values are plotted. Bar in A, 20 µm.

In both control and dynamitin-overexpressing Cos7 cells, Cy3-Tfn-labeled particles exhibited mostly short-range oscillations(<0.5 µm; Table 1; Ghosh and Maxfield, 1995; Schrader and Schroer,unpublished results). These movements did not appear to be actomyosinbased, because they were not inhibited by treatment of cells withthe actin poison, latrunculin A, or the broad-spectrum myosininhibitor butanedione monoxime (our unpublished results). Longer-range(>0.5-µm), presumably microtubule-based, movements were occasionallyobserved in control cells, but these were not common, and rarerin cells overexpressing dynamitin (Table 1).

Inhibition of Early to Late Endosome Traffic and Motility

Unlike early endosomes, late endosomes undergo robust motility that is thought to use the dynein/dynactin motor complex. Totest this hypothesis directly, control and dynamitin-overexpressingCos7 cells were loaded with Cy3-labeled $alpha$ ₂-M. This classic endocyticmarker (Willingham and Pastan, 1978) enters cells by receptor-mediateduptake but, unlike Tfn, dissociates from its receptor in earlyendosomes (Yamashiro et al., 1989) and is trafficked to late endosomes.At early times of observation (0-25 min) Cy3- $alpha$ ₂M appeared in structuresthat resembled those labeled with FITC-Tfn (Figure 5A, middle).After ~25 min, the fluorescent particles in control cells hada variety of sizes and shapes, including round structures (0.1-4.5µm diameter) and branched or elongated tubules (0.7-4 µm long).These translocated over long distances (up to 6 µm) in curvedor straight trajectories (motility is quantified Table 1; Schraderand Schroer, unpublished results). Although the labeled structureswere most abundant in the center of the cell, they moved in alldirections (inward, outward, and parallel to the cell margin),and many moved bidirectionally, suggesting that they were poweredby both plus and minus end-directed motors. Motility persistedfor >1 h.

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Figure 5. Analysis of endocytic trafficking in control and dynamitin-overexpressing cells. (A) HeLa cells were labeled with Cy3- $alpha$ ₂-M for 10 min and then chased for 5 min and fixed with paraformaldehyde. The same cells were then stained for early endosomes (EEA1; left) and overexpressed dynamitin (right); $alpha$ ₂-M staining is shown in the middle. (B) As in A, except the cells were chased for 1 h after the $alpha$ ₂-M pulse to allow the probe to traffic to late endosomes. After fixation, the cells were stained for EEA1 (left) and LBPA (right); $alpha$ ₂-M staining is shown in the middle. For A and B, the small panels to the right are 3× magnification views of the boxed areas; cells overexpressing HA-dynamitin are marked with asterisks. Arrows in A indicate early endosomes that also stain for $alpha$ ₂-M. (C) Qualitative analysis of $alpha$ ₂-M uptake and accumulation. Transfected Cos7 cells were labeled for 20 min and then fixed immediately (left panel) or chased for 90 min and then fixed (right panel). The fluorescence intensity (bright, dim, or no label) of $>=$ 150 cells was assessed for each condition. (D) Subcellular distribution of endosomes loaded with Tfn or $alpha$ ₂-M. Transfected HeLa cells were loaded with fluorescent tracers, fixed immediately, and then scored for endosome location. Central, random, and peripheral indicate the site of the most predominant staining. Similar results were obtained in Cos7 cells (our unpublished results). (E) Analysis of endosome pH in transfected, live Cos7 cells. pH was measured by fluorescence ratio imaging (Kim et al., 1996

). Data were acquired from at least two different coverslips in two independent experiments. Dynamitin overexpressers were identified by staining with anti-HA (A, B, and D) or pAb dynamitin (C) or by Golgi morphology (E).

As expected, cells overexpressing dynamitin showed a dramatically different labeling pattern from controls. After a shortpulse of $alpha$ ₂-M, the intensity (Figure 5C, left) and morphologyof labeled particles were similar to control cells, suggestingthat uptake and delivery to early endosomes was unaffected. However,the labeled endosomes were either randomly distributed or concentratedat the periphery (Figure 5D), and many colocalized with earlyendosomes stained for EEA1 (Figure 5A). For the first hour ofobservation, neither the randomly distributed nor peripheral structuresmoved to an appreciable degree (Table 1). Importantly, outward(i.e., plus end-directed) movements were not observed. Similareffects on Cy3 $alpha$ ₂-M uptake, localization, and particle motilitywere seen in most cells overexpressing the dynamitin N terminus(our unpublishedresults).

After a 60-min chase, most dynamitin-overexpressing cells still contained detectable amounts of $alpha$ ₂-M, like the controls. Theprobe now colocalized with late endocytic markers (Figure 5B),suggesting that delivery to late endosomes had occurred. However,some cells were not labeled, and an increased percentage showedreduced levels of accumulation (Figure 5C). Because nearly allcells took up the probe originally, this finding suggested thatearly to late endocytic trafficking might be subtly perturbed.If traffic to late endosomes were slowed, $alpha$ ₂-M in early endosomesmight have more opportunities to be released from thecell.

In most dynamitin-overexpressing cells Cy3- $alpha$ ₂-M accumulated in long-lived structures that colocalized with late endosome markers.To further characterize this compartment, we measured its lumenalpH (Figure 5E). For this analysis, cells were allowed to trafficFITC- $alpha$ ₂-M to late endosomes for $>=$ 30 min. In both dynamitin-overexpressingand control cells, the labeled structures had a lumenal pH inthe range of 5.0-5.5, the expected value for late endosomes. Themean pH increased slightly with increasing chase time, but thepH distribution was always the same as in controls, and the broadrange of values obtained made any differences statistically insignificant.Acidification of endosomes containing $alpha$ ₂-M did not appear to beappreciably altered by dynamitinoverexpression.

Although dynamitin overexpression has profound effects on endosome localization and motility, our findings suggest it doesnot dramatically alter compartment function. Cells can still takeup endocytic probes and recycle them to the surface or deliverthem to late endosomes with the appropriate pH. This may not besurprising, because both early and late endosomes in dynamitin-overexpressingcells are near the cell periphery, which would obviate the needfor long-range movement between the two compartments. However,some cells showed reduced accumulation of $alpha$ ₂-M, suggesting thatearly-to-late endocytic traffic might be slowed. To determinethe effects on trafficking of another endocytic cargo, we examinedthe cells' susceptibility to VSV, a virus that must be endocytosedand delivered to a low pH compartment to be infective. Virus infectionis inhibited by endosome alkalization or conditions that interferewith endocytic trafficking, such as inhibition of coatomer functionby mutation (Daro et al., 1997) or antibody microinjection (Whitneyet al., 1995). For the present experiments, Vero cells were incubatedwith a temperature-sensitive VSV strain (ts-O45 VSV), and infectionefficiency was measured by staining for newly synthesized viralglycoprotein (ts-O45-G; Figure 6A). Cells were infected at roomtemperature and then maintained at the restrictive temperature(39.5°C), which causes ts-O45-G to accumulate in the ER (Bergmannet al., 1981). After infection for 1 h, only ~10% of Vero cellsmicroinjected with the dynamitin expression construct showed detectablelevels of ts-O45-G in the ER, compared with 80% of cells microinjectedwith a control vector. Cells containing dynamitin introduced bytransfection were also resistant to virus infection; only ~25%of the cells had detectable levels of ts-O45-G protein expressioncompared with 80% of the transfection controls (Figure 6B). Todetermine whether virus infection was completely blocked or justdelayed, cells were infected for longer times (1.5-2 h at 20°C)or at a higher temperature (1-2 h at 37°C). Under these conditions,nearly 100% of control cells were infected. An increase (to 60-80%;Figure 6B) in infected dynamitin-overexpressing cells was alsoobserved. This supports our hypothesis that trafficking throughthe endocytic pathway is delayed but not completely inhibitedby dynamitin overexpression.

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Figure 6. Effect of dynamitin overexpression on virus infection and protein export. (A) Vero cells transfected with dynamitin (top panels) or GFP (bottom panels) were infected with ts-O45 VSV for 1 h at 17-20°C and maintained at 39.5°C to retain VSV-G protein in the ER. After 3 h, cells were fixed and stained for dynamitin (HA; top left) or GFP (bottom left) and VSV-G protein (right top and bottom, mAb P5D4 and polyclonal serum). Cells overexpressing HA-dynamitin are marked with asterisks. Bar, 20 µm. (B) Quantitation of infection. Vero cells were microinjected (gray bars) with HA-dynamitin or Sar1p (a yeast rab) or transfected (black bars) with HA-dynamitin, GFP, or $beta$ -gal and infected for 1 h at room temperature (RT; 17-20°C). Control cells that received no DNA (white bar) were infected in parallel. Cells were stained, and the percent expressing both the exogenous protein and ts-O45-G protein was determined. At least 220 dynamitin-overexpressing cells, in four independent experiments, were counted for each condition. Sar1p overexpression was documented on two separate coverslips in a single experiment. The GFP bar shows data from GFP and $beta$ -gal transfections. In the remaining five black bars, cells were infected for 1 h at RT, 1.5 h at 20°C, 2 h at 20°C, 1 h at 37°C, or 2 h at 37°C.

Association of Dynactin and CLIP-170 at Microtubule Ends

Our data verify that the dynein/dynactin motor is a major contributor to microtubule-based movement of endosomes. However,live cell imaging studies reveal that, for several minutes afterentering the cell, endocytic probes in early ("sorting") endosomesremain fairly stationary and do not undergo long-range, microtubule-dependenttranslocations (Ghosh and Maxfield, 1995; Schrader and Schroer,unpublished results). This delay most likely reflects the timerequired for the probe to transit to the appropriate endosomalsubcompartment (endocytic carrier vesicle or late endosome). However,once this has occurred, an additional mechanism is required tobind the endosome to the microtubule track. CLIP-170 has beenproposed to serve the initial docking role, because this proteincan interact with both endosomes (Pierre et al., 1992) and thedistal ends of microtubules (Rickard and Kreis, 1990). Short arraysof CLIP-170 treadmill at microtubule plus ends as they grow towardthe periphery (Perez et al., 1999), providing a potential mechanismfor attachment of peripheral endosomes and other structures (Dujardinet al., 1998).

The p150^Glued subunit of dynactin contains a CLIP-170-related microtubule-binding motif that may contribute to dynein processivityby transiently stabilizing the enzyme-cargo link (King, and Schroer,2000). Given the structural similarities of CLIP-170 and p150^Glued (Pierre et al., 1992) and their overlapping roles in endosome-microtubuleinteractions, these two proteins may work in concert at microtubuleplus ends. CLIP-170 might promote the formation of a nonmotile,microtubule-endosome complex, which would first recruit dynactinand then dynein. As a first test of this model, we compared thesubcellular localizations of CLIP-170 and dynactin in HeLa cells.Previous dynactin localization studies showed a fine, punctatestaining throughout the cell and accumulation at centrosomes (Gillet al., 1991; Paschal et al., 1993; Waterman-Storer et al., 1995;Holleran et al., 1996). Some of this staining colocalizes withCLIP-170 (Vaughan et al., 1999). In double-labeling studies, wealso observed dynactin staining that colocalized with CLIP-170in short linear arrays in the cell periphery (Figure 7, a andb).

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Figure 7. Effects of dynamitin overexpression on colocalization of CLIP-170 and dynactin at microtubule ends. (a and b) Control cells costained for CLIP-170 and dynactin (Arp1). (c and d) High-magnification view of two cells overexpressing dynamitin at a low level showing staining of peripheral microtubule ends. (e and f) High-level dynamitin overexpression (asterisks in e marks overexpressing cells). HeLa cells were stained for CLIP-170 (pAb 55, a; mAbs 2D6 and 4D3, c and e), dynactin (Arp1 mAb 45A, b) or dynamitin (pAb anti-HA, d and f). All were fixed with MeOH. Bars, 20 µm. Magnification in insets a1-b3, 4×.

Both CLIP-170 and dynactin p150^Glued are able to bind microtubules directly via their N-terminal microtubule binding sites (Pierreet al., 1992; Waterman-Storer et al., 1995). According to ourmodel, CLIP-170 binds microtubules first. To test this hypothesis,we overexpressed different dynactin subunits and determined theireffects on CLIP-170 localization. If intact dynactin were required,dynamitin overexpression would be expected to alter CLIP-170 distribution.When overexpressed at low levels, dynamitin colocalized with CLIP-170along microtubules (Figure 7, c and d). Even high-level dynamitinoverexpression had no detectable effect on CLIP-170 at microtubuleplus ends (Figure 7e and f), corroborating a recent report (Vaughanet al., 1999). These results indicate that CLIP-170 plus end bindingdoes not require intactdynactin.

Dynamitin overexpression causes p150^Glued to dissociate from dynactin's Arp1 backbone (Echeverri et al., 1996). The released p150^Glued may still be able to interact with potential binding partners,including microtubules. In dynamitin-overexpressing cells, p150^Glued is still seen at microtubule ends (Vaughan et al., 1999). Whenp150^Glued by itself is overexpressed in cells, it binds microtubules alongtheir length (Waterman-Storer et al., 1995; Figure 8b). CLIP-170in these cells is still present in peripheral, linear arrays (Figure8a), suggesting that CLIP-170 binds microtubule plus ends independentlyof p150^Glued.

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Figure 8. Effects of p150^Glued and CLIP-170 overexpression on CLIP-170 and dynactin localization. (a and b) p150^Glued overexpression. (c-f) Effects of wt CLIP-170 overexpression on p150^Glued (c and d) and Arp1 (e and f) staining. (g and h) Overexpression of CLIP-170 $Delta$ T (lacking the C-terminal domain that contains the metal-binding motif). HeLa cells were stained for CLIP-170 (pAb 55, a and e; 2D6 and 4D3, c; anti-myc mAb 9E10, g) or dynactin (p150^Glued: mAb 150.1, b; pAb 150^Glued, d and h; Arp1: mAb 45A, f). All were fixed with MeOH. Bars, 20 µm. Inset magnifications, 2×.

Parallel experiments were performed to determine whether CLIP-170 overexpression affected dynactin localization. At low levels,overexpressed CLIP-170 forms small microtubule-associated structures(Figure 8e), and at higher levels, CLIP-170 accumulates in patchyaggregates (Figure 8c; (Pierre et al., 1994). These structuresalso stained for dynactin subunits (p150^Glued, Figure 8d; Arp1, Figure 8f). The localizations of the Golgicomplex, late endosomes, and lysosomes were normal in cells overexpressingCLIP-170 (Figure 9). This suggests that the actions of dyneinand dynactin contribute more significantly than CLIP-170 to thefinal distributions of these organelles.

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Figure 9. Effects of CLIP-170 overexpression on Golgi complex, late endosome, and lysosome distributions. HeLa cells were fixed with MeOH and stained with Abs to (a and c) CLIP-170 (pAb 55), (b) galactosyl transferase, and (d) CD63 (a LAMP family member; mAb 1B5). Bar, 20 µm.

In addition to its microtubule-binding domain, CLIP-170 contains a metal-binding motif (Pierre et al., 1992) that is implicatedin cargo interactions (Pierre et al., 1994; Dujardin et al., 1998).Deletion of the protein domain containing this motif yields amutant species that can still bind microtubules but does not accumulatein aggregates (Pierre et al., 1994; Figure 8g). The mutant proteindoes not recruit dynactin (Figure 8h), suggesting that the putativecargo-binding domain is required for the interaction. Moreover,dynactin is no longer detected in linear stretches at microtubuleplus ends. Quantitative determination of the prevalence of theperipheral, linear dynactin staining revealed it in nearly allof cells in the control population (97%; n = 191) but in onlya minority (18%; n = 38) of those overexpressing the mutant CLIP-170species. This reinforces the idea that CLIP-170 binds microtubuleplus ends independently of dynactin and again suggests that theCLIP-170 putative metal-binding domain contributes to dynactininteractions.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Our data provide new insights into the roles of dynein, dynactin, and CLIP-170 in endosome function. The clear but limitedeffects of dynamitin overexpression on endocytic trafficking refineour understanding of the contributions of microtubule-based movementto this process. CLIP-170 and dynactin colocalize at microtubuleplus ends, and binding is found to be CLIP-170 dependent, suggestinga hierarchy of binding. We have also identified the highly conserveddynamitin N terminus as a novel potential dynein-binding element.On the basis of our findings, we propose a series of molecularinteractions that may underlie endosome docking and movement.Endosome-associated CLIP-170 provides the initial link to microtubulesand recruits dynactin, which then binds dynein. Once dynein isbound and/or activated, CLIP-170 releases its grip on the microtubule,and long-range endosome motilitybegins.

The discovery that overexpression of the dynamitin N terminus perturbs endomembrane dynamics without affecting dynactin structurewas unexpected. Although p150^Glued is the only dynactin subunit that has been shown to bind dyneindirectly (reviewed by Allan, 1996; Schroer, 1996; Holleran etal., 1998), our results suggest that dynamitin may also play arole. p150^Glued and dynamitin are tightly associated within the projecting dynactinsidearm (Eckley et al., 1999) that is proposed to serve as thedynein-binding site. Dynamitin may stabilize the dynein-dynactininteraction by binding dynein directly. We find (Quintyne et al.,1999) that overexpression of different dynactin subunits can havea variety of effects, including Golgi complex and endosome dispersion,disorganization of the interphase microtubule array, and disruptionof dynactin structure. Dynamitin induces all these effects, whereasother dynactin subunits such as p150^Glued disrupt Golgi structure and microtubule organization withoutaffecting dynactin integrity. These overexpressed dynactin subunits,as well as the p150^Glued released by dynamitin overexpression, most likely perturb dynactinfunction by competing for binding sites on dynein or cargo. Thedynamitin N terminus may act in a similarmanner.

We suspect that the immediate effect of dynamitin overexpression is to inhibit dynein-based movement selectively, allowingplus end-directed movement to predominate for a short time, insupport of a previous hypothesis (Burkhardt et al., 1997). However,we observe no plus end-directed particle movements in dynamitin-overexpressingcells, suggesting that, at steady state, kinesin and/or kinesin-relatedprotein-based motility is also inhibited. Late endosomes and lysosomesmight possess a latent microtubule plus end binding activity (e.g.,CLIP-170) that would explain their microtubule-dependent retentionat the periphery (Burkhardt et al., 1997; Harada et al., 1998).Regardless of the mechanism for endosome relocalization, our resultssuggest that cells overexpressing dynamitin have arrived at anew steady-state condition in which endosome movement has stopped.Under normal conditions, overall membrane flux is kept in balanceso that export parallels import (Steinman et al., 1976). The bidirectionalmovement of individual organelles (e.g., lipid droplets) is alsoheld in balance, because motility in both directions is alteredin parallel when cells are subjected to physiological (Hamm-Alvarezet al., 1993) or genetic manipulation (Welte et al., 1998). Endosomemovements may be subject to similar controls. Current models ofthe mechanism underlying coordinated organelle movement invokea shared motor receptor (Sheetz et al., 1989; Vallee and Sheetz,1996), although other mechanisms are possible. The use of dynamitinoverexpression and other dynein-selective inhibitors should proveuseful in further studies of this importantquestion.

Our results suggest the additional intriguing possibility that endosome function is governed by a control mechanism that linkstrafficking with compartment architecture. Precedent is seen intwo trafficking-defective Chinese hamster ovary cell lines thatexhibit distinct endocytosis phenotypes (McGraw et al., 1993;Daro et al., 1997). Both show peripheral accumulations of earlyand late endosomes without any obvious alteration to microtubules.Similar endosome rearrangements are seen in chloroquine-treatedchick embryo fibroblasts (Lippincott-Schwartz and Fambrough, personalcommunication). Apparently, disruption of endocytic traffic andendosome rearrangement are tightly coupled. Although the primarydefect is different from cells overexpressing dynamitin (e.g.,the ldlF cell line encodes a mutant $epsilon$ -COP; Daro et al., 1997),mutant Chinese hamster ovary cells show alterations in late endosomefunction similar to those we observe. Endocytic cargoes such asVSV (Daro et al., 1997) and ricin (McGraw et al., 1993) do notpass from acidic endosomal compartments to the cytoplasm, anddelivery of epidermal growth factor to lysosomes is impaired (Daroet al., 1997). In dynamitin-overexpressing cells and in mutantcell lines, short-range cycling of material between early endosomesand the plasma membrane continues. Late endosomal membranes maybe induced to cycle in parallel when traffic is disrupted. Theperturbation of normal mechanisms for forward or inward movement(e.g., budding or dynein-driven motility) might then allow theendosomal compartments participating in these loops to accumulatein the cell periphery near sites ofuptake.

Early events in the endocytic pathway, such as ligand uptake and receptor recycling, are found to occur normally in dynamitin-overexpressingcells. However, trafficking to late endosomes is slowed. Undernormal conditions, microtubules have been proposed to expeditetransfer of material from early to late endosomes, perhaps viaendocytic carrier vesicles (Gruenberg et al., 1989). Why then,in cells in which these compartments are near each other, shouldendocytic traffic be impaired? One possibility is that dynein-basedmotility is required to transport endocytic vesicles in the peripherythrough actin-rich cortex (Marsh and Bron, 1997). The spatialsegregation that results from microtubule-based movement may alsobe required to maintain the distinct functions of different endocyticcompartments (Gruenberg and Maxfield, 1995; Mellman, 1996). Endosomesthat have been relocated to the cell periphery may fuse promiscuouslywith each other, which would result in membrane mixing unlessbalanced by sorting and retrieval mechanisms. Early and late endosomemarkers remain distinct in dynamitin-overexpressing cells, indicatingthat the two compartments are not completely randomized. However,inappropriate exchange of functionally important components orinhibitory factors not examined here might lead to the traffickingdelays weobserve.

Early and late endosomes are both highly pleiomorphic organelles, yet no clear relationship between structure and functionhas been established. The membrane deformations induced by microtubulemotor activity may, in fact, contribute to membrane fusion. Inpure lipid bilayer systems, high degrees of membrane curvaturefacilitate fusion (Chernomordik, 1996). The enhancement of earlyand late endosome content mixing in vitro seen in the presenceof microtubules (Aniento et al., 1993) may be another reflectionof thisphenomenon.

Whatever other roles it may play in trafficking, it is clear that the dynein/dynactin motor is critical for the translocationof endosomal membranes on microtubules. What remains an open questionis how endosomes switch from the short-range, oscillatory movementsseen early on to the long-range, bidirectional translocationsseen at later times. The discovery that dynactin colocalizes withCLIP-170 at microtubule ends suggests an order of assembly ofthe microtubule-endosome complex. Microtubules extending intothe periphery may contact an endosome and become docked via CLIP-170.Once the endosome is tethered in this manner, CLIP-170 can recruitdynactin. At this point, dynactin may simply provide a dynein-bindingsite, or it may transiently stabilize the endosome-microtubuleassembly via its own cargo- and microtubule-binding sites. Toswitch from this stable binding configuration to one that allowsmotility, the CLIP-170-microtubule link must be severed, perhapsby phosphorylation. This model provides many hypotheses to betested in futurestudies.

	ACKNOWLEDGMENTS

We thank C. Crego and N. Jeangunat for technical assistance, Dr. M. Gomez for the microinjection studies, M. Cheng,Dr. M. Eckley, Dr. S. King, and N. Quintyne for Figure 3, andN. Quintyne for the Nile Red results. Thanks to Drs. J. Gruenberg,H.-P. Hauri, A. Helenius, A. Linstedt, M. Marsh, I. Mellman, O.Rosorius, K. Simons, and T. Suganuma for antibodies and Drs. W.Balch, M. Gomez, W.J. Nelson, J. Rickard, and G. Warren for expressionvectors. We thank members of the Kreis and Schroer laboratoriesfor helpful discussions and valuable comments on the manuscript.C.V. was supported by a European Molecular Biology Organizationlong-term fellowship and Telethon grant 411/bi; D.M.W. was supportedby a Howard Hughes Undergraduate Summer Research Fellowship anda Johns Hopkins University Provost's Award; M.S. was supportedby a grant from the Deutsche Forschungsgemeinschaft; T.E.K. wassupported by the Fonds Nationale Suisse and the Canton de Genève;and T.A.S. was supported by National Institutes of Health grantsGM-44589 and DK-44375 and a Lucile and David Packard Fellowshipfor Science andEngineering.

	FOOTNOTES

Present addresses: Department of Experimental Medicine, Anatomy Section, University of Genova, Via De Toni 14, 16132 Genova,Italy;

^§ Medical Scientist Training Program, Washington University School of Medicine, 660 S. Euclid Avenue, St. Louis, MO 63110;

Institute for Cytobiology, Clinic of Philipps-University Marburg, Robert-Koch-Strasse 5, 35037 Marburg, Germany;

^¶ Department of Anatomy and Neuroscience, Washington University School of Medicine, 660 S. Euclid Avenue, St. Louis, MO 63110;

^# The Institute for Genomic Research, 9712 Medical Center Drive, Rockville, MD20850.

^** Corresponding author. E-mail address: schroer{at}jhu.edu.

ABBREVIATIONS

Abbreviations used: $alpha$ ₂-M, $alpha$ ₂-macroglobulin; Arp1, actin-related protein 1; $beta$ -gal, $beta$ -galactosidase; CMV, cytomegalovirus; DMB, dimethyl BODIPY; EEA1, early endosomal antigen 1; ER, endoplasmic reticulum; EST, expressed sequence tag; GFP, green fluorescent protein; HA, influenza hemagglutinin; LBPA, lysobisphosphatidic acid; Tfn, transferrin; TGN, trans-Golgi network; ts-O45-G, vesicular stomatitis virus glycoprotein, Orsay 45 temperature-sensitive strain; VEDIC, video-enhanced differential interference contrast; VEFM, video-enhanced fluorescence microscopy; VSV, vesicular stomatitis virus; VSV-G, VSV glycoprotein; wt, wild type.

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