The Golgi Complex Is a Microtubule-organizing Organelle

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Vol. 12, Issue 7, 2047-2060, July 2001

The Golgi Complex Is a Microtubule-organizing Organelle

Karine Chabin-Brion,^* Jérôme Marceiller,^* Franck Perez, Catherine Settegrana,^* Anne Drechou,^* Geneviève Durand,^* and Christian Poüs^*

^*Laboratoire de Biochimie et de Biologie Cellulaire, EA 1595, Faculté de Pharmacie, 92296 Châtenay-Malabry Cedex, France; and Centre National de la Recherche Scientifique UMR 144, Institut Curie Section Recherche, 75248 Paris Cedex 05, France

Submitted March 13, 2001; Revised March 13, 2001; Accepted April 26, 2001
Monitoring Editor: Suzanne R. Pfeffer

	ABSTRACT

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

We show that the Golgi complex can directly stimulate microtubule nucleation in vivo and in vitro and thus behaves as a potentmicrotubule-organizing organelle in interphase cells. With theuse of nocodazole wash-out experiments in hepatic cells, we foundthat the occurrence of noncentrosomal, early stabilized microtubulesis highly correlated with the subcellular localization of Golgimembranes. With the use of in vitro reconstituted microtubuleassembly systems with or without cytosol, we also found that,in contrast to centrosomally attached microtubules, the distalends of Golgi-attached microtubules are remotely stabilized ina way that requires additional cytosolic component(s). Finally,we demonstrate that Golgi-based microtubule nucleation is directand involves a subset of $gamma$ -tubulin bound to the cytoplasmic faceof theorganelle.

	INTRODUCTION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

In interphase cells, the microtubule (MT) network plays a major role in membrane dynamics and organelle localization. In thiscontext, the interaction between the Golgi complex and the MTnetwork has been extensively studied. The Golgi apparatus colocalizeswith the minus ends of MTs, which are usually associated withthe centrosome (for review see Kreis et al., 1997; Thyberg andMoskalewski, 1999). This localization actually results from anequilibrium between two contradictory movements that have beenunraveled with the use of MT-depolymerizing drugs and probablyoccur on MT subpopulations with different dynamics. The dispersalof Golgi elements occurs along stable MTs after depolymerizationof the most labile MT population (Minin, 1997), whereas theirreclustering involves newly assembled MTs (Ho et al., 1989). Thesecontradictory movements of Golgi elements are mediated by distinctmolecular motors. Consistent with earlier findings by Feiguinet al. (1994), who found that the expression of kinesin antisenseoligonucleotide rendered the Golgi apparatus more compact, microinjectionof antikinesin antibodies inhibited Golgi dispersion along stable,nocodazole-resistant MTs (Minin, 1997). Conversely, the centrallocalization of the Golgi apparatus involves cytoplasmic dynein(Corthésy-Theulaz et al., 1992; Fath et al., 1994; Burkhardtet al., 1997; Harada et al., 1998). It is also worth noting that,in addition to the kinesin-mediated disruption of the centralGolgi complex during MT depolymerization, the dispersion of Golgielements also relies on the reconstitution of mini Golgi stacksat endoplasmic reticulum (ER) exit sites (Cole et al., 1996; Storrieet al., 1998). Such data on the scattering and the reclusteringof the Golgi complex have led to the view that Golgi membranesundergo an intimate relationship with MTs and especially witha population of nocodazole-resistant, stable MTs. Stable MTs arecharacterized by the occurrence of posttranslationally modifiedtubulin $---$ especially detyrosinated and acetylated tubulin (for review,see MacRae, 1997), which is thought to accumulate in stable MTsbecause of their longer half-lives, but does not influence MTstability in vivo (Schulze et al., 1987; Khawaja et al., 1988;Webster et al., 1990). Interestingly, not only MT stability influencesGolgi localization, but Golgi membranes may reciprocally influenceMT stabilization. Such an idea has been suggested by the spatialand temporal colocalization of detyrosinated or acetylated MTsand Golgi or trans-Golgi network (TGN) membranes that occurs innocodazole wash-out experiments (Skoufias et al., 1990; Burgesset al., 1991; Thyberg and Moskalewski, 1993). After nocodazoleremoval, tubulin acetylation not only occurs radially from thecentrosome (just like detyrosination does), but it is also foundin discrete cytoplasmic locations (Bulinski et al., 1988). Theoccurrence of scattered acetylated MTs close to Golgi elementsduring the MT repolymerization process (Thyberg and Moskalewski,1993) was also reminiscent of the occurrence of stable, noncentrosomalMTs during MT repolymerization in MDCK cells (Bré et al., 1987).Altogether, these data suggested that Golgi membranes could beinvolved in the assembly and in the early stabilization of a subsetof noncentrosomal MTs. Consistently, it has been shown that otherbiological membranes such as fish melanophore pigment granulesand fish fibroblast membranes can readily nucleate MTs in vivo(Rodionov and Borisy, 1997; Kaverina et al., 1998) or that theapical membrane of polarized epithelial cells participate in theorganization of the interphase MT network (Meads and Schroer,1995). Regarding MT stabilization, the recent identification ofthe cis-Golgi network (CGN)-associated MT-associated protein GMAP-210,and its association with a hyperstable population of detyrosinatedMTs are also in favor of Golgi-mediated MT stabilization (Infanteet al., 1999).

In this study, we show that in addition to the centrosome, the Golgi apparatus is a potent MT-organizing organelle. In vivo,scattered Golgi elements stimulate the assembly of noncentrosomalMTs upon recovery from nocodazole treatment. We further show that,in contrast to the high level of dynamics found in centrosomalMTs, Golgi-based MTs are stabilized early. The in vitro reconstitutionof MT assembly by purified Golgi membranes also showed that MTstabilization required additional cytosolic factor(s) and thatMT nucleation directly involved Golgi-bound $gamma$ -tubulin.

	MATERIALS AND METHODS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Antibodies and Chemicals

Native (clone DM1A) and acetylated (clone 6-11B-1) anti- $alpha$ -tubulin, anti- $gamma$ -tubulin (clone GTU-88), rabbit anti-mouse IgG, anti-rabbitand anti-mouse IgG FITC, and TRITC conjugates, nocodazole, saponin,and protein A Sepharose were purchased from Sigma Chemical Co.(St. Louis, MO). Anti- $beta$ -tubulin mAb (clone DM1B) was purchasedfrom Amersham-Pharmacia Biotech (Uppsala, Sweden). Various markersof the Golgi were used including an mAb to rat mannosidase II(clone 53FC3) from Berkeley Antibody Co. (Richmond, CA), antialbuminimmunserum raised in rabbits as previously described (Biou etal. 1984), anti-GM130 Golgi matrix protein (Transduction Laboratories,Lexington, KY), and anti-TGN38, kindly provided by Dr. GeorgeBanting, Department of Biochemistry, School of Medical Sciences,University of Bristol, UK (Reaves and Banting, 1992). For thedetection of centriolar proteins, we used the mAb (clone GT335)to polyglutamylated tubulin (Eddé et al., 1990), kindly providedby Pr. Philippe Denoulet (Centre National de la Recherche Scientifique,FRE2219 Université Paris VI) and a polyclonal antibody to centrin-3(Middendorp et al., 1997), kindly provided by Dr. Michel Bornens(Centre National de la Recherche Scientifique, Unité Mixte deRecherche 144, Institut Curie, Paris), who also provided the nucleo-centrosomalextract used as a positive control. FITC-conjugated anti-mouseFab fragments were purchased from Jackson ImmunoResearch (WestGrove, PA). Okadaic acid was from Life Technologies (Rockville,MD). Phosphocellulose-purified porcine brain tubulin was preparedas described by Walker et al. (1988).

Cell Culture and Nocodazole Treatments

WIF-B cells were cultured in F12 Coon's-modified medium (Sigma Chemical Co.) supplemented with 5% FCS (Dutscher, Rungis, France)and HAT mixture (10⁵ M hypoxantine, 4 ×10⁷ M aminopterine and 1.5 × 10⁵ M thymidine; Polylabo, Strasbourg, France). Cells were confluentand normally polarized 8-10 d after plating at a initial densityof 7000 cells/cm². Fao cells were cultured in the same medium as WIF-B cells withoutthe HAT mixture. NIH-3T3 cells were cultured on glass coverslipsin DMEM medium supplemented with 10%FCS.

Nocodazole and brefeldin A (BFA) were diluted to 10 µM in culture medium, starting from a 10 mM stock solution in dimethylsulfoxide or in methanol, respectively. To achieve total MT depolymerization,cells were treated with nocodazole for 10 h. The effectivenessof such treatment has been verified previously in WIF-B cells(Poüs et al., 1998) and in Fao cells (our unpublishedresults).

Immunofluorescence

WIF-B cells were cultured on glass coverslips, and after appropriate treatments were rinsed three times with 0.1 M PBS, pH7.4, at room temperature and then fixed and permeabilized withmethanol at $-$ 20°C for 5 min. All antibody incubations and washeswere performed in PBS. Cells were incubated with primary antibodiesfor 1 h at 37°C, washed three times, and incubated (1 h, 37°C)with FITC-conjugated antibodies or a mixture of FITC- and TRITC-conjugatedantibodies for single- or double-labeling experiments, respectively.Because secretory albumin is a convenient marker of the Golgiapparatus in untreated WIF-B cells (Cassio et al., 1991; Shankset al., 1994; Poüs et al., 1998), we verified by double immunofluorescencelabeling that during Golgi dispersal and nocodazole wash-out,albumin and mannosidase II, a resident enzyme of the medial Golgi,remained colocalized in WIF-B and Fao cells (our unpublished results).To perform double-labelings with two mouse monoclonal antibodies,cells were first incubated with the first antibody (1 h, 37°C),washed three times, and incubated (2 h, 37°C) with FITC-conjugatedanti-mouse Fab fragments. After three washes, immune complexeswere fixed with methanol ( $-$ 20°C, 5 min), and then cells were incubatedwith the second antibody (always the anti- $alpha$ -tubulin) for 1 h at37°C, washed three times, and incubated (1 h, 37°C) with anti-mouseTRITC conjugate. After three washes, the coverslips were mountedin Slow Fade (Molecular Probes, Eugene,OR).

To assess MT stability after 15-min nocodazole wash-out, two protocols were used: first, a dilution-induced depolymerizationassay in which cells were incubated (5 times, 1 min, 37°C) inHEPES-buffered medium (100 mM HEPES, 2 mM MgCl₂, 1 mM EGTA, pH6.9) containing 200 µg/ml saponin and then fixed in methanol andprocessed for the immunofluorescence labelings of acetylated tubulinand secretory albumin; and second, after the 15-min wash-out periodafter nocodazole treatment, cells were subjected to a second nocodazoletreatment (20 min, 10 µM, 37°C), rinsed, and then fixed in coldmethanol and processed for the immunofluorescence labelings oftubulin and secretoryalbumin.

Confocal microscopy was performed with the use of a TCS 4D laser scanning microscope (Leica, Heidelberg, Germany). Unlessotherwise specified, the images shown are the superimpositionof consecutive optical sections taken over the whole cell height,the distance between two consecutive optical sections being lessthan the z resolution of the microscope (delta z < 0.5 µm). Tomake sure that no artifactual juxtapositions resulted from theprojection of the organelles imaged in distant confocal planes,each optical section was first examined separately to observethe spatial associations between MTs and Golgi fragments. If MTswere found not to be in contact with Golgi fragments, the adjacentupper and lower optical sections were also examined to detectjuxtaposed Golgifragments.

Experiments in Permeabilized Cells

Morphologically intact Golgi membranes from rat liver were prepared according to Hui et al. (1998). This method routinelygave a 80- to 120-fold enrichment of the galactosyl transferaseactivity compared with the homogenate. Microtubule dynamics wasreconstituted in detergent-extracted NIH 3T3 fibroblasts accordingto Saoudi et al. (1998) with the after modifications. SubconfluentNIH-3T3 cells cultured on glass coverslips (22 × 22 mm) were permeabilizedin PEM buffer (100 mM PIPES, 1 mM EGTA, 1 mM MgCl₂, pH 6.9) supplementedwith 0.05% Triton X-100 (3 times, 1 min, 37°C). Cells were thenkept at 4°C for 3 d to achieve cold-induced MT depolymerization.Cytosol from interphase NIH-3T3 cells was prepared as describedexcept that cells were sonicated instead of being permeabilizedwith Triton. Permeabilized cells were incubated for 30 min at37°C with 35 µl cytosol, 5 µM okadaic acid, 2.5 µM phosphocellulose-purifiedporcine brain tubulin, and an ATP-regenerating system. When appropriate,20 µM nocodazole was added for 30 min before cells were rinsedtwice with 1 ml of warm PEM buffer and fixed with methanol ( $-$ 20°C,3 min). MTs and Golgi membranes were immunolabeled with antibodiesto $alpha$ -tubulin and rat serum albumin, respectively. Samples wereexamined in a Leica DMLB microscope with a 100×objective.

In Vitro Experiments

Golgi membranes were incubated with 10 µM purified porcine brain tubulin in the presence of 1 mM GTP for 15-30 min at 37°C.After rapid fixation with 0.25% glutaraldehyde, Golgi membraneswere centrifuged (20,000 × g, 30 min) through a 15% sucrose cushionon glass coverslips, postfixed in methanol ( $-$ 20°C, 4 min), andsubjected to immunofluorescencelabeling.

Salt-wash experiments were conducted as follows: Golgi membranes were first incubated in 2 M KCl for 1 h on ice. After a rapidspin down of Golgi membranes, the pellet was resuspended in PEMbuffer, extensively washed with PEM, and put on the top of a sucrosegradient comprised of a 1.3 M sucrose cushion and a 0.25 M sucroseoverlayer, both buffered with 100 mM, pH 6.7, phosphate, and supplementedwith 5 mM MgCl₂. When appropriate, salt-washed Golgi membraneswere gently resuspended and agitated for 1 h at room temperaturein WIF-B cytosol. After centrifugation, the Golgi was washed twicewith PEM buffer, then resuspended in PEM, and used in the MT-assemblyassay as described above. WIF-B cytosol was obtained by sonicationof trypsinized cells resuspended 1:1 in PEM buffer. The lysatewas ultracentrifuged (30 min, 200,000 × g, 4°C), and the supernatantwas frozen in liquid nitrogen and kept at $-$ 80°C until use. Immunodepletionof $gamma$ -tubulin was performed by adding 15 µl of the GTU-88 antibodyto 35 µl WIF-B cytosol diluted 20 times with PEM buffer. Aftergentle rotation (2 h, room temperature), the immune complexeswere harvested by three consecutive incubations with 25 µl ofprotein A-Sepharose beads precoated with rabbit anti-mouse IgGs(2 h, room temperature). After concentration with the use of Ultrafreecentrifugal filter devices (Millipore Corp., Bedford, MA), thecytosolic extract was controlled for the absence of detectable $gamma$ -tubulin by Western blotting beforeuse.

	RESULTS

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

Stable Acetylated MTs Occur in the Close Vicinity of Golgi Fragments Early after Nocodazole Wash-out

As a prerequisite to the study of the assembly of new MTs during nocodazole wash-out experiments, we first validated the experimentalconditions in which all the MTs from interphase cells were completelydepolymerized. Total depolymerization is essential because, dependingon the cell type, stable MTs exhibit such a slow turnover thatthey may remain intact during a whole interphase (Webster et al.,1987). It was achieved in both WIF-B and Fao cells by a 10-h treatmentwith 10 µM nocodazole. We have shown previously that tubulin acetylationis the only posttranslational modification of stable MTs in WIF-Bcells (Poüs et al., 1998). The same was true in Fao cells, exceptfor very rare cases in which detyrosinated tubulin was observedin isolated cells. We thus labeled acetylated tubulin to followstable MT disassembly and repolymerization during nocodazole treatmentand wash-out,respectively.

First, as described previously in fibroblasts (Thyberg and Moskalewski, 1993), we observed that in Fao and WIF-B hepatic cellsscattered acetylated MTs reformed in the vicinity of Golgi elements.In untreated Fao (Figure 1A) and WIF-B cells (Figure 1B), theGolgi complex was observed as a compact, juxtanuclear organelle,in an acetylated MT-rich region. In WIF-B cells, the Golgi wasclose to the apical membrane, which delimitates bile canaliculi(Figure 1B, arrowhead). After nocodazole treatment, the Golgicomplex was disrupted into numerous elements scattered in thecytoplasm (Figure 1, C and D). In the same conditions, acetylatedMTs could not be detected, except for two centriolar spots (Figure1, C and D), which colocalized with $gamma$ -tubulin (our unpublishedresults). Fifteen minutes after nocodazole removal, two populationsof acetylated MTs were found. Some acetylated MTs were radiallyorganized, most likely around the centrosomes, whereas anotherpopulation appeared to be scattered in the cytoplasm (Figure 1,E and F). Interestingly, these small MT segments were juxtaposedto Golgi elements (Figure 1, E-H). These MT segments did not followa particular direction in the cytoplasm, nor did cell polarityseem to influence their subcellular localization because theirdistribution appeared relatively uniform in both cell lines. Additionally,WIF-B cells did not exhibit a higher density of such MTs neartheir apical membranes. To quantify the juxtaposition of MT segmentsto Golgi elements, we measured the distribution of the distancesbetween the two organelles on images of individual confocal slicestaken at shorter wash-out times than shown in Figure 1, so thatproximity could be interpreted as clearly as possible. When anMT was found to be isolated, the two adjacent slices were alsotaken in consideration to determine the distance of the closerGolgi element. Table 1 shows that the distances measured after5- or 10-min wash-outs were predominantly shorter than 0.2 µm.Because we measured a 1.5-µm mean distance between scattered Golgielements, this data confirms that the proximity between Golgiand MTs was not due to random juxtapositions.

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Figure 1. Acetylated MTs reform in the close vicinity of Golgi fragments. Fao rat hepatoma cells (A, C, E, and G) and WIF-B polarized hepatic cells (B, D, F, and H) were treated without (A and B) or with (C-F) 10 µM nocodazole for 10 h, washed twice with cold culture medium, and incubated at 37°C in nocodazole-free medium for 15 min (E, F, G, and H). Cells were then fixed and processed for double immunofluorescence labeling with the use of antibodies to acetylated tubulin (green) and secretory albumin (red). All cells were examined by confocal microscopy. The images shown in A-F are the superimposition of serial optical sections acquired over the whole cell height (delta z = 0.5 µm). In G and H, two images with a shorter depth of field (made by superimposing 3 consecutive optical sections) were extracted from the indicated regions in E and F, respectively. The arrowhead indicates a bile canaliculus between adjacent WIF-B cells. Scale bar, 10 µm.

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Table 1. Frequency distribution of the distances between Golgi elements and MT segments

To test if these newly assembled acetylated MTs were actually stable, two approaches were used after recovery from nocodazoletreatment. We first triggered the depolymerization of dynamicallyunstable MTs in Fao (Figure 2A) and WIF-B (Figure 2B) cells byperforating the plasma membrane with saponin. The second approachconsisted in treating cells a second time with nocodazole to depolymerizehighly dynamic MTs (Figure 2, C and D). Although centrosomal MTswere acetylated, they did not resist the second nocodazole treatmentin both cell lines (Figure 2, C and D) or dilution in WIF-B cells(Figure 2B). In contrast, and in both conditions, the scatteredacetylated MT population was still present, indicating that mostof the early regrown MTs juxtaposed to Golgi fragments were morestable than centrosomally assembled acetylated MTs.

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Figure 2. Newly formed acetylated MTs associated with Golgi elements are stable. Nocodazole wash-out experiments were conducted as described in Figure 1 on Fao (A and C) and WIF-B cells (B and D). Cells were either permeabilized with HEPES-buffered medium containing 0.2 mg/ml saponin (A, B) or incubated again with 10 µM nocodazole for 20 min at 37°C (C and D). After fixation, cells were subjected to double immunofluorescence labeling of acetylated tubulin (green) and secretory albumin (red). All cells were examined by confocal microscopy. The images are the superimposition of consecutive optical sections taken over the whole cell height (delta z = 0.5 µm). Scale bar, 10 µm.

The Occurrence of Noncentrosomal Acetylated MTs Is Golgi Dependent

Because they were not radially organized, the scattered acetylated MT segments that occurred close to Golgi fragments werelikely to be noncentrosomal. However, it was still possible thatthese MTs would be centrosomally attached and that they wouldbe stabilized and acetylated on their distal domains because ofcontact with Golgi elements. To discriminate between these twohypotheses, we repeated nocodazole wash-out experiments, visualizingboth nonmodified and acetylated tubulin. The centrosomal MT populationwas composed of a mixture of acetylated (as observed in Figure1, E and F) and unmodified MTs, which were longer and more abundantin Fao (Figure 3A) than in WIF-B cells (Figure 3B). As for discreteMT acetylation, the superimposition of consecutive confocal slicesclearly shows that the scattered acetylated MT segments belongedto longer MTs, which were not connected with the centrosomes.These noncentrosomal MTs were randomly oriented in the cytoplasmand were acetylated at only one end (Figure 3, A and B). The factthat noncentrosomal MT repolymerization did not occur more frequentlybelow the apical membrane than in the rest of the cytoplasm ofWIF-B cells also indicates that cell polarity did not influencethe early building of the MT network in hepatic cells.

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Figure 3. Scattered acetylated MTs belong to noncentrosomal microtubules. Fao rat hepatoma cells (A) and WIF-B polarized hepatic cells (B) were subjected to the same nocodazole wash-out experiments as described in Figure 1. After fixation, acetylated tubulin (center panels) and $alpha$ -tubulin (left panels) were visualized by immunofluorescence on a confocal microscope. The images shown are the superimposition of consecutive optical sections acquired over the whole cell height (delta z = 0.5 µm). A bile canaliculus (b.c) is indicated between two adjacent WIF-B cells. Scale bar, 10 µm.

To evaluate further whether the subcellular localization of noncentrosomal MTs correlates with that of Golgi membranes, MTswere depolymerized by the combined actions of cold and nocodazoleto prevent the dispersion of the Golgi complex (Turner and Tartakoff,1989), and then the temperature was shifted back to 37°C for 15min after nocodazole removal to allow MT assembly. As shown forWIF-B cells (Figure 4B), the Golgi remained essentially in a centrosomallocation, although very small Golgi fragments also occurred throughoutthe cytoplasm and were probably rebuilt from the ER (Cole et al.,1996; Storrie et al., 1998). In these conditions, there was adramatic drop in the amount of noncentrosomal MTs (Figure 4B)compared with cells in which nocodazole treatment was performedat 37°C (Figure 4A). The sites of noncentrosomal MT assembly thusappeared to follow the position of Golgi elements, strongly suggestingthat Golgi elements are actually involved in the assembly of thenoncentrosomal MT population. The fact that newly assembled MTsgathered around the centrosome/Golgi location in these conditionsruled out the possibility that other organelles distributed throughoutthe cytoplasm such as the ER or mitochondria could be involvedin the occurrence of noncentrosomal MTs. Regarding early endosomesthat are localized in the same area as the Golgi, we also checkedthat upon nocodazole wash-out, previously internalized fluorescenttransferrin did not colocalize with Golgi and TGN markers (ourunpublished results). To further study the dependence of noncentrosomalMT assembly on the localization of Golgi membranes, we testedwhether the nucleating capacity of Golgi elements can be redistributedto the ER upon BFA treatment. Additional experiments were conductedin which cells were treated with BFA before MT depolymerizationand nocodazole wash-out. In Figure 4C where cells were subjectedto tubulin and albumin labeling, noncentrosomal MTs still occurred,whereas albumin was redistributed back into the ER. As shown inFigure 4D, however, the Golgi matrix protein GM130, which redistributesto the CGN and/or to the intermediate compartment upon BFA treatment(Nakamura et al., 1995), occurred as discrete elements that wereclosely associated with noncentrosomal MTs. Consistent with thisobservation, the distribution of the distance measurements betweenMTs and GM130 locations was very similar to that described inTable 1 (our unpublished results), suggesting that in these conditions,MTs might regrow off the intermediate compartment that containedGolgi matrix proteins.

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Figure 4. The subcellular localization of newly assembled microtubules is correlated with Golgi membrane location. WIF-B polarized hepatic cells were pretreated (C, D) or not with 10 µM BFA for 1 h at 37°C and then subjected to MT depolymerization by 10 µM nocodazole at 37°C for 6 (C and D) or 10 h (A). In B, MT depolymerization was conducted at 4°C for 2 h. Cells were then allowed to recover from nocodazole treatment at 37°C for 15 min. After fixation, cells were either subjected to the double-immunofluorescence labeling of $alpha$ -tubulin (left panels) and secretory albumin (middle panels of A-C) or to that of $alpha$ -tubulin and GM130 (middle panel of D). The images are the superimposition of equidistant optical sections acquired by confocal microscopy over the whole cell height (delta z = 0.5 µm). Scale bars, 10 µm.

Purified Golgi Stimulate MT Assembly and Stabilization In Vitro

The previous experiments gave highly correlative results, suggesting that Golgi stacks could promote the assembly of noncentrosomalMTs and stabilize them in vivo, but there were two issues withthis approach. First, we could not formally exclude the hypothesisthat these peripheral stable MTs could be due to the severingof centrosomal MTs followed by treadmilling (Rodionov and Borisy,1997) before capture and stabilization by Golgi elements. Second,it was impossible to determine by in vivo experiments whetherMT stabilization was direct or not and whether MT stabilizationand assembly resulted from the samemechanism.

We thus conducted MT assembly and stabilization experiments in a system slightly modified from that described by Saoudi etal. (1998), in which interphase-like MT dynamics was reconstitutedin detergent-extracted cells. In this system, MT dynamics werereestablished in permeabilized NIH 3T3 cells with the use of amixture of detergent-free fibroblastic cytosol, an ATP-regeneratingsystem, and a protein phosphatase inhibitor. Because detergentextraction in PEM buffer temporarily preserved cellular MTs fromdepolymerization, we further modified this protocol to completelydepolymerize the MT network in the cold before testing MT reassemblyand stability in the presence of purified Golgi. When incubatedfor 30 min with purified Golgi, this system allowed both the formationof Golgi-based MTs (Figure 5A) and that of centrosomal MT asters(Figure 5B). When the MT assembly period was followed by a 30-mintreatment with 20 µM nocodazole, centrosomal asters, as expected,completely depolymerized (Figure 5D). In contrast, MTs surroundingGolgi elements resisted nocodazole treatment (Figure 5C) in avery similar way as MTs attached to Golgi elements did in vivo.This indicates that, in conditions that mimic as much as possiblewhat happens in living cells, including the high level of MT dynamicsfound in centrosomal asters, exogenous Golgi was still capableof stimulating MT assembly and actually stabilized MTs.

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Figure 5. Golgi membranes nucleate and stabilize microtubules when added to a permeabilized cell system in which interphase microtubule dynamics were reconstituted. NIH-3T3 fibroblasts cultured on glass coverslips were detergent-extracted with 0.05% Triton X-100 in PEM buffer, rinsed extensively, and kept at 4°C for 3 d. Permeabilized cells were then incubated for 30 min at 37°C with detergent-free, autologous cytosol containing 2.5 µM tubulin, 5 µM okadaic acid, an ATP-regenerating system, and purified Golgi. In C-D, 20 µM nocodazole was added for 30 more min at 37°C. After two rinses with warm PEM buffer, samples were fixed with methanol ( $-$ 20°C, 4 min) and processed for the double-immunofluorescence labeling of tubulin (left panels) and albumin (right panels). Depending on the distribution of Golgi elements and cells on the coverslip, images of Golgi-containing or control (containing extracted cells) regions are shown as indicated. Scale bar, 10 µm.

To test whether Golgi-mediated MT assembly and stabilization are direct or not, we further simplified the above system tofinally keep purified rat liver Golgi, purified tubulin, and GTP.After assembly periods of 15 or 30 min, samples were fixed, centrifugedonto glass coverslips, and subjected to the double-immunofluorescencelabeling of Golgi markers and $alpha$ -tubulin. As expected, no spontaneousMT assembly occurred in the absence of Golgi membranes (Figure6, A and B). When the system was supplemented with purified Golgi,MTs assembled, increasing in length as a function of time (Figure6, C-F). It is worth noting that Golgi elements exhibited significanttubulin labeling over the whole membrane (Figure 6, C and E),even when they were incubated without tubulin (our unpublishedresults). As measured from six independent experiments (overalln = 300), only 65 ± 8% of the labeled Golgi elements actuallyallowed MT assembly. By performing labelings of TGN38 or mannosidaseII instead of GM130 (Figure 6, E and F, insets), we checked thatboth markers were generally detected whatever the effectivenessof Golgi elements in nucleating MTs, suggesting that this effectivenessdid not result from the enrichment in a Golgi subcompartment.To know further whether the MTs assembling around Golgi elementswere also stabilized by the organelle, 10 µM nocodazole was addedfor 15 min after a 15-min assembly period. In these conditions,all the MTs were depolymerized (Figure 6, G and H), indicatingthat these MTs were highly dynamic in contrast with the in vivosituation and with what happened in the presence of cytosol andATP in the permeabilized cell system. This experiment demonstratedthat Golgi elements are directly capable of stimulating MT assembly,and, together with the data shown in Figure 5, it indicated thatadditional factor(s) are required to stabilize them. Adding theATP-regenerating system and the protein phosphatase inhibitorto the minimal in vitro assembly system did not allow Golgi-basedMTs to further resist nocodazole treatment (our unpublished results),indicating that cytosolic component(s) are required to specificallystabilize Golgi-based MTs.

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Figure 6. Purified Golgi membranes promote the assembly of microtubules in vitro but have no microtubule-stabilizing effect. Purified Golgi membranes were added (C-H) or not (A and B) to 0.1% purified porcine brain tubulin and 1 mM GTP in PEM buffer. After 15- or 30-min incubations at 37°C, followed (G and H) or not (A-F) by the addition of 10 µM nocodazole for 15 more min as indicated, samples were fixed by a 20-fold dilution with 0.25% glutaraldehyde in PEM buffer and sedimented although a 15% sucrose cushion onto glass coverslips. After postfixation in methanol ( $-$ 20°C, 4 min), samples were processed for the immunofluorescence labeling of $alpha$ -tubulin (left panels) and GM130 (right panels, B-H), TGN38 or Mannosidase II (F, insets) as indicated. Scale bar, 10 µm

$gamma$ -Tubulin Is Involved in the Nucleation of Golgi-based MTs

To further understand the mechanism of Golgi-based MT assembly, we first tested the specificity of our minimal in vitro assemblyassay, considering the possibility that Golgi preparations mightbe systematically contaminated with centrosomes. To this end,purified Golgi membranes were analyzed by Western blotting forthe presence of centrosomal markers, as well as for that of tubulinsto confirm their presence on the Golgi from a biochemical pointof view. As expected, both $alpha$ - (Figure 7A) and $beta$ -tubulin (our unpublishedresults) were detected in Golgi samples. The Golgi preparationalso contained significant amounts of $gamma$ -tubulin (Figure 7A). Froma quantitative point of view, although the specific concentrationof $alpha$ -tubulin in the Golgi was identical to that measured in ahepatocyte lysate, $gamma$ -tubulin was slightly enriched (~2 times)in the Golgi preparation. As shown in Figure 7B, the centriolarmarker centrin-3 (Middendorp et al., 1997) was not detected insignificant amounts in the Golgi compared with a nucleo-centrosomalextract. Consistently, neither was polyglutamylated tubulin (Eddéet al., 1990) detected in Golgi samples (our unpublished results).To evaluate from Figure 7B the specificity of $gamma$ -tubulin bindingto Golgi membranes, a $gamma$ -tubulin to centrin ratio was measuredin the Golgi and in the nucleo-centrosomal extract. This ratiowas ~25 times higher in the Golgi than in the nucleo-centrosomalextract, thus confirming that the presence of $gamma$ -tubulin on Golgimembranes was not due to a high level of contamination by centrosomes.

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Figure 7. $gamma$ -Tubulin is peripherally associated with Golgi membranes. (A) Purified rat liver Golgi membranes (50 µg of total proteins) and increasing amounts of rat hepatocyte lysate were analyzed by 9% SDS-PAGE followed by Western blotting for the presence of $alpha$ - and $gamma$ -tubulin. Band intensities were analyzed by densitometry to estimate the enrichment of Golgi membranes in both markers relative to the lysate (see the text). (B) The amount of centriolar material was measured in Golgi samples compared with a nucleo-centrosomal extract (C+N) by SDS-PAGE (9 and 15% for $gamma$ -tubulin and centrin-3, respectively), followed by electrotransfer onto polyvinyl difluoride membranes, postfixation with 0.2% glutaraldehyde (only for centrin), and immunorevelation. Densitometric measurements of band intensities were used to evaluate the ratios of $gamma$ -tubulin to centrin signals and to allow a comparison between the Golgi and the C+N extract (see the text). (C) Purified Golgi was incubated for 30 min at 37°C with 0.1% tubulin and 1 mM GTP. After fixation with 0.25% glutaraldehyde, samples were centrifuged onto glass coverslips and postfixed with methanol before the double-labeling of $alpha$ - and $gamma$ -tubulins as indicated. Scale bar, 10 µm.

Even though it has been shown to be largely distributed in the cytosol (Moudjou et al., 1996), $gamma$ -tubulin was only known toplay a role at the level of the MTOC. The binding of $gamma$ -tubulinto Golgi membranes was quite unexpected, but it also suggesteda mechanism for Golgi-based MT nucleation. We thus checked that $gamma$ -tubulin was actually present at the surface of those Golgi elementsthat nucleate MTs. As shown above for other Golgi markers (seeFigure 6), $gamma$ -tubulin was readily detected on both nucleating andnonnucleating Golgi elements (Figure 7C). We further tried toaddress the function of Golgi-bound $gamma$ -tubulin in two ways. First,we used a monoclonal anti- $gamma$ -tubulin (clone GTU-88) directed againstthe N-terminal domain of the protein (amino acids 38-53), whichis involved in the MT-nucleating activity of $gamma$ -tubulin in centrosomes(Joshi et al., 1992). Figure 8A shows that the preincubation ofGolgi membranes with GTU-88 completely inhibited in vitro MT nucleation,whereas preimmune mouse IgGs did not affect MT assembly. Second,as GTU-88 binding at the surface of the Golgi might have alsosterically blocked any other neighboring proteins involved inMT assembly, we tried to overcome this limitation in the followingway. We initially found that a 2 M KCl wash caused the completeloss of $alpha$ -, $beta$ -, and $gamma$ -tubulin from purified Golgi, confirmingthat they were peripherally associated with the organelle. Accordingly,its MT-nucleating property was completely abolished (Figure 8B).Interestingly, all the attempts to reconstitute $gamma$ -tubulin bindingfailed when we used the proteins that had been stripped off theGolgi membranes. We then reconstituted the interaction of $gamma$ -tubulinwith salt-washed Golgi membranes by incubating them with a WIF-Bcytosolic extract similar to that used in the semiintact cellsexperiments (see Figure 5). In these conditions, $gamma$ -tubulin didrebind to the Golgi (Figure 8C) and that binding resulted in therecovery of the MT-nucleating property of Golgi membranes. Whena $gamma$ -tubulin-depleted extract was used instead of crude cytosol,no MT nucleation could be observed (Figure 8C). It is also worthnoting that $gamma$ -tubulin immunodepletion had to be quantitative aslow residual concentrations of $gamma$ -tubulin were still able to restorethe MT-nucleating capacity. Altogether these data indicate thatperipherally bound $gamma$ -tubulin is actually involved in nucleatingMTs on Golgi membranes.

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Figure 8. $gamma$ -Tubulin is involved in the nucleation of Golgi-based MTs. (A) As indicated, purified Golgi was preincubated either with anti- $gamma$ -tubulin or with preimmune mouse IgGs for 1 h at 37°C and then used in the in vitro MT assembly assay. Samples were processed for the immunofluorescence labeling of $alpha$ -tubulin. (B) Purified rat liver Golgi was washed as indicated with 2 M KCl and then rinsed three times in PEM buffer before being assayed for the presence of tubulins or to be used in the in vitro MT assembly assay. Samples were analyzed for the presence of tubulins by Western blotting, as described in Figure 7. After the in vitro MT assembly assays, samples were subjected to the immunofluorescence labeling of $alpha$ -tubulin. (C) Salt-washed Golgi membranes were incubated (1 h, room temperature) with crude WIF-B cytosol or cytosol that was immunodepleted of $gamma$ -tubulin and then rinsed twice in PEM buffer and either analyzed by Western blot for the presence of peripherally bound $gamma$ -tubulin or used in the in vitro MT assembly assay, followed by the immunofluorescence labeling of $alpha$ -tubulin. Scale bar, 10 µm.

	DISCUSSION

TOP ABSTRACT INTRODUCTION MATERIALS AND METHODS RESULTS DISCUSSION REFERENCES

We found that the Golgi complex is involved in organizing a subset of stable MTs independently from the centrosome in interphasecells. Upon nocodazole removal after complete MT depolymerizationand Golgi breakdown, a population of acetylated MTs occurred innoncentrosomal cytoplasmic locations that were highly correlatedwith those of Golgi elements. By contrast with the labile populationof centrosomal acetylated MTs, this noncentrosomal MT subset wasstabilized early. We further showed that purified Golgi membranesexhibited an intrinsic MT nucleating property, whereas they neededadditional cytosolic component(s) to achieve MT stabilization.Having found that $alpha$ -, $beta$ -, and $gamma$ -tubulins are bound to Golgi membranes,we showed that peripherally associated proteins were requiredfor performing Golgi-based MT nucleation and more specificallythat $gamma$ -tubulin itself was involved in the nucleatingprocess.

We showed in vitro that Golgi membranes are directly responsible for the assembly of noncentrosomal MTs. This means that ourin vivo observations were likely not to result from the severingand release of centrosomal MTs (Baas and Joshi, 1992; Yu et al.,1993; Keating et al., 1997; Vorobjev et al., 1997) or even spontaneouscytoplasmic assembly, followed by treadmilling or migration enbloc (Rodionov and Borisy, 1997; Vorobjev et al., 1997; Yvon andWadsworth, 1997; Tucker et al., 1998) until they were capturedand stabilized by scattered Golgi elements. Because the reconstitutionof mini-Golgi stacks at ER exit sites actively participates inthe dispersion of the Golgi complex after nocodazole-mediatedMT depolymerization (Cole et al., 1996; Storrie et al., 1998),the ER would also have been a likely candidate for stimulatingnoncentrosomal MT assembly. This possibility was clearly ruledout because the vast majority of newly assembled MTs followedthe Golgi when the organelle was kept in a central location duringMT depolymerization. Interestingly, the results we obtained uponBFA treatment suggested that the MT-assembling properties of theGolgi are not linked to glycosyltransferases or to other proteinsthat are redistributed back to the ER but rather to proteins likeGM130, which are retained in the intermediate compartment/CGNin these conditions. Our data thus identify the Golgi as a centralorganelle involved in the assembly of a subset of stable MTs.Other membrane organelles such as fish melanophore pigment granules(Rodionov and Borisy, 1997) might be involved in organizing MTsin the absence of centrosome. These data, together with the factthat pinocytic vesicles organize actin bursts upon internalization(Merrifield et al., 1999), support the view that some membraneorganelles are not solely organized in a passive way by the cytoskeletonbut that they actively participate in the organization of cytoskeletalstructures.

We found that significant amounts of $alpha$ - and $beta$ -tubulins are bound to the Golgi. A direct anchoring of palmitoylated tubulinin membranes has been demonstrated in platelets (Caron, 1997;Ozols and Caron, 1997), but such an anchoring was unlikely tobe involved in the case of Golgi membranes because tubulins wereall lost after salt-wash. The binding of tubulin to Golgi membranesmight also be due to an interaction with Golgi-resident proteinssuch as $beta$ -1,4-galactosyltransferase (Yamaguchi and Fukuda, 1995).Another possibility would be that very short tubulin polymersmight interact with molecular motors constitutively bound to Golgimembranes (Vaisberg et al., 1996; for review, Hirokawa et al.,1998) or with $gamma$ -tubulin, which we identified as a key moleculeinvolved in nucleating Golgi-based MTs. $gamma$ -Tubulin could be recruitedfrom the cytosolic pool to promote MT nucleation, but, by analogywith what happens in the centrosomes, it should be organized ina nucleating complex such as a ring complex (Zheng et al., 1995)that may cap MT minus ends (Wiese and Zheng, 2000). The moleculesthat actually recruit and/or organize $gamma$ -tubulin on Golgi membranesstill remain to be identified. The assembly of $gamma$ -tubulin ontocentrosomes being mediated by cytoplasmic dynein in a MT-dependentmanner (Young et al., 2000), one might even speculate that cytoplasmicdynein, which was also identified on Golgi membranes (Vaisberget al., 1996; Roghi and Allan, 1999), might be needed to someextent for assembling and/or docking $gamma$ -tubulin on theGolgi.

At the level of the centrosome, a sequential model has emerged in which MTs are first nucleated on $gamma$ -tubulin-containing complexesand then released and anchored on distinct sites (Quintyne etal., 1999; Mogensen et al., 2000). A similar model might alsoapply for the Golgi complex in which the Golgi-associated MAPGMAP-210 that was shown to bind both the minus end of MTs andCGN membranes (Infante et al., 1999) would be a good docking candidate.Additionally, the MT-stabilizing effect of Golgi membranes andthe fact that GMAP associates with a subset of stable MTs in vivo(Infante et al., 1999) might also fit well with this hypothesis.In this respect, the in vitro system we used to reconstitute theMT-stabilizing effect only reproduced plus-end dynamics, whichis necessary and sufficient to restore the sensitivity of MTsto nocodazole (Saoudi et al., 1998). This also is consistent withthe fact that MTs might be anchored to Golgi membranes by theirminus ends, with their plus ends being free to grow and shrink.A puzzling question would remain, however: how can MT plus endsbe remotely stabilized when the minus ends binds to Golgi membranes?Insoluble cytoplasmic structures such as intermediate filamentsmight be involved, even though they are not indispensable forthe reclustering of Golgi elements around the centrosome (Ho etal., 1989). More likely, soluble cytosolic factor(s) might specificallyrecognize Golgi-bound MTs and participate directly in their earlystabilization or be needed to activate a Golgi-bound molecularmotor that would slide toward the plus end and contribute to itsstabilization. Such a hypothesis would be supported by the recentfinding that detyrosinated MTs are stabilized by an ATP-sensitive,plus-end cap that resembles kinesins (Infante et al., 2000).

Although our data provide many evidence for the capability of Golgi membranes to assemble MTs and stabilize them, the physiologicalrole of such properties is stillunclear.

The simplest situation in which cell physiology resembles nocodazole wash-out conditions is the postmitotic reclustering ofGolgi elements in the pericentrosomal area. Astral MTs seem indispensablefor the reclustering of the organelle in a central location (Shimaet al., 1998), but intermediate steps in this process might involvethe capture of Golgi-attached MTs in the centrosomal area to facilitatethe reclustering process. Such a model would require Golgi MTsto exhibit reverse polarity or would be quite complicated in termsof molecular motor regulation, because Golgi reclustering is dyneindependent (Corthésy-Theulaz et al., 1992; Fath et al., 1994,Burkhardt et al., 1997; Harada et al., 1998). This would be ina way similar to the behavior of chromosomes during mitosis becausethey have the possibility to directly nucleate MTs in additionto their capture by centrosomal MTs (Carazo-Salas et al., 1999).Another possibility would be that Golgi-attached MTs participatein the local merger of postmitotic Golgi elements before theirfinal reclustering. It is known from nocodazole wash-out experimentsthat each Golgi fragment is not directed to the centrosomal regionbut that local merger occurs before final reclustering (Ho etal., 1989). The role of Golgi-based MTs would be to organize locallythe neighboring mini-stacks into bigger structures that wouldfinally be targeted to the centrosomal area. Because Golgi membranescan actually stabilize MTs, one could propose that the Golgi complexplays a key role in the differentiation of the MT network by specificallystabilizing a MT subset on exit from mitosis. Indeed, Golgi elementsalso codistribute with a subset of early acetylated MTs duringtelophase, before the occurrence of detyrosinated MTs (Thybergand Moskalewski, 1993). After the growing evidence for the functionalspecialization of distinct classes of MTs, depending on theirstability (Mizuno and Singer, 1994; Nagasaki et al., 1994;Gurlandand Gundersen, 1995; Tanaka et al., 1995; Minin, 1997; Poüs etal., 1998), our understanding of the molecular events that leadto MT stabilization has also grown regularly (for review see Gundersenand Cook, 1999). However, even though some biochemical data showthat the small GTPase RhoA stabilizes only a subset of MTs (Cooket al., 1998), virtually nothing is known about how a specificsubset of MTs might be selectively recognized before stabilization.Because postmitotic Golgi fragments are reclustered around thecentrosome along astral MTs (Shima et al., 1998), Golgi elementsmight serve as a differentiation device to identify the futuresubset of stable MTs in interphasecells.

During the interphase, MTs are required for performing effective protein trafficking toward the cell surface or back to theendoplasmic reticulum (for review see Cole and Lippincott-Schwartz,1995; Bloom and Goldstein, 1998). Dynamic and stable MTs are specializedin mediating specific transport steps (Mizuno and Singer, 1994;Poüs et al., 1998), which may involve various molecular motors,often localized on Golgi membranes (Vaisberg et al., 1996; forreview see Hirokawa, 1998). The way such specialized motor proteinsspecifically interact with the appropriate target membranes isstill an open question but may be related to the regulation ofmembrane traffic, as suggested by the example of rabkinesin-6,which binds the small GTPase Rab6 involved in Golgi-to-ER retrogradetransport (Echard et al., 1998). This example illustrates theprobable need for specific GTPases, specific molecular motorsand appropriate MTs to operate a given membrane transport stepin vivo. From this perspective, our results also suggest thatupon the activation of the transport machinery, Golgi membranesmight assemble and perhaps stabilize the appropriate MTs insteadof depending on centrosomally attached MTs for the vectorizationof membrane carriers. This would allow the cell to define prioritytracks to use for efficient vesicular transport. Because the Golgicomplex does behave as a potent organizer and a differentiatingdevice of a stable subset of MTs, it will be interesting now toaddress the corresponding molecular mechanisms in more detail.In this perspective, the in vitro systems that we developed willbevaluable.

	ACKNOWLEDGMENTS

The authors are grateful to Dr. Doris Cassio for her enthusiastic encouragements; to Drs. Thu Phung-Koskas, Germain Trugnan,Michèle Maurice, and Tounsia Ait Slimane for critical advicein discussing the experimental work; and to Drs. George Banting,Michel Bornens, and Philippe Denoulet for providing cell extractsand antibodies. The authors are also grateful to the InstitutFederatif de Recherche 02 "Cellules épithéliales" from the InstitutNational de la Santé et de la Recherche Medicale, Faculté deMédecine Xavier Bichat, 75018 Paris, for the availability ofthe confocal microscope. This work was supported by a grant fromthe "Institut de Recherches InternationalesServier."

	FOOTNOTES

Corresponding author. E-mail address: christian.pous{at}cep.u-psud.fr.

ABBREVIATIONS

Abbreviations used: BFA, brefeldin A; CGN, cis-Golgi network; ER, endoplasmic reticulum; MT, microtubule; TGN, trans-Golgi network.

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