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The mitotic spindle mediates inheritance of the Golgi ribbon structure
Correspondence to Joachim Seemann: joachim.seemann{at}utsouthwestern.edu
The mammalian Golgi ribbon disassembles during mitosis and reforms in both daughter cells after division. Mitotic Golgi membranes concentrate around the spindle poles, suggesting that the spindle may control Golgi partitioning. To test this, cells were induced to divide asymmetrically with the entire spindle segregated into only one daughter cell. A ribbon reforms in the nucleated karyoplasts, whereas the Golgi stacks in the cytoplasts are scattered. However, the scattered Golgi stacks are polarized and transport cargo. Microinjection of Golgi extract together with tubulin or incorporation of spindle materials rescues Golgi ribbon formation. Therefore, the factors required for postmitotic Golgi ribbon assembly are transferred by the spindle, but the constituents of functional stacks are partitioned independently, suggesting that Golgi inheritance is regulated by two distinct mechanisms.
© 2009 Wei and Seemann
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During cell division, the single Golgi ribbon needs to be segregated into the two daughter cells. To achieve partitioning, the Golgi fragments at the onset of mitosis, and later reforms in each daughter cell (for review see Lowe and Barr, 2007). Two different mechanisms have been proposed for the partitioning of the Golgi. In one view, Golgi membranes are absorbed into and partitioned with the ER (Zaal et al., 1999). The second view argues that the Golgi remains distinct from the ER and that the two compartments are inherited independently (Bartz and Seemann, 2008). In this scenario, the spindle has been proposed as the machinery responsible for Golgi partitioning based on the observed accumulation of Golgi membranes at the spindle poles (Shima et al., 1998), although a pool of membranes is dispersed throughout the cytoplasm (Jesch et al., 2001).
To elucidate the role of the spindle in Golgi partitioning, we established an assay in which the entire spindle is segregated into only one daughter cell. Upon division, a Golgi ribbon reformed in the karyoplasts, whereas the stacked cisternae were scattered throughout the cytoplasts. We could rescue ribbon assembly in the cytoplasts by microinjecting the Golgi extract together with tubulin or by lowering the division temperature, at which partial spindle materials were transferred into the cytoplasts. We propose that Golgi factors required for ribbon assembly rely on the spindle for partitioning, but functional stacks are inherited independently. This reveals two levels of regulation underlying Golgi inheritance. Coupling of these factors with the spindle would ensure that daughter cells receive the information to assemble the Golgi ribbon, which is vital for cellular functions that require polarized secretion and directional migration.
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Results and discussion |
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TopAbstractIntroductionResults and discussionMaterials and methodsReferences |
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To eliminate the possibility that the scattered Golgi in the cytoplasts might be caused by cell death, we followed both karyoplasts and cytoplasts by video microscopy. The cytoplasts survived on average 36 h after division and, in some cases, were still alive and seemingly healthy when corresponding karyoplasts underwent a second round of cell division.
The scattered Golgi and the absence of microtubules in the cytoplasts are reminiscent of cells treated with nocodazole, which causes the Golgi ribbon to fragment into stacks that are dispersed throughout the cell (Shima et al., 1998). Our EM analysis revealed that the Golgi in both karyoplasts and cytoplasts was stacked with an average of 3.4 ± 0.7 (karyoplast; n = 22) and 3.3 ± 0.6 (cytoplast; n = 23) cisternae per stack (Fig. 3, A and B). The cisternae were stacked to a comparable extent and separated by 11.8 ± 3.8 (karyoplast) and 12.9 ± 3.7 nm (cytoplast). To determine whether the stacks were polarized, we took advantage of a well-established fluorescence microscopy method (Shima et al., 1997). PtK1 cells stably expressing the medial/trans-Golgi enzyme NAGT I–GFP were induced to divide asymmetrically and immunolabeled for GFP and the cis-Golgi marker GM130 (n = 15). In these triple-labeled cells, the GFP fluorescence was first overlaid with the anti-GFP signal (Fig. 3, C and D) and was then overlaid with the anti-GM130 signal (Fig. 3, E and F). The anti-GFP staining served as a control, showing a complete overlap with the GFP fluorescence (Fig. 3, C and D). In contrast, the cis–anti-GM130 signal in the karyoplasts was found adjacent to the medial/trans-GFP fluorescence with only a partial overlap (Fig. 3 E), suggesting that the ribbon in the karyoplasts preserved a cis-to-trans polarity. A similar segregation pattern was observed in the cytoplasts (Fig. 3 F). Together with our EM data, we conclude that the scattered Golgi in the cytoplasts is stacked and polarized.
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In principle, the lack of a Golgi ribbon in the cytoplasts could be explained by two different mechanisms. First, the failure in ribbon assembly might be a result of the absence of microtubules in the cytoplasts because microtubules are essential to establish a Golgi ribbon. In this case, reformation of microtubules should restore the ribbon. Alternatively, the scattered Golgi stacks in the cytoplasts might be caused by the exclusion of the factors required for ribbon assembly (i.e., ribbon determinants). Ribbon determinants may associate with the spindle and are therefore not transferred to the cytoplasts. Supplying these factors should rescue ribbon formation. To distinguish between these two possibilities, we injected the missing materials into the cytoplasts and examined the Golgi morphology. Injection of tubulin resulted in a microtubule network (Fig. 4 C), demonstrating that the cellular environment in the cytoplasts supports microtubule polymerization (Pelletier et al., 2000). However, the overall organization of Golgi stacks remained scattered (n = 14, five independent experiments; Fig. 4 B), indicating that the microtubules in the cytoplasts are not sufficient to reassemble a ribbon. Therefore, additional factors might be required but were presumably segregated along with the spindle into the karyoplasts. Because these factors may associate with Golgi membranes, we extracted rat liver Golgi (RLG) membranes with the nonionic detergent n-octylglucoside and removed the detergent by dialysis. Injection of Golgi extract alone had no effect (n = 12, four independent experiments; Fig. 4 F), but Golgi extract together with tubulin restored a ribbon (n = 8, five independent experiments; Fig. 4 J) as well as a microtubule network (Fig. 4 K). Thus, the factors required for ribbon assembly are located on the Golgi.
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If the ribbon determinants are partitioned with the spindle, incorporation of parts of the spindle and its associated proteins into the cytoplasts should rescue ribbon formation. We followed asymmetrical cell division induced at lower temperature (32°C) and found that spindle positioning was dramatically altered, presumably caused by effects on microtubule dynamics (Fig. S2, available at http://www.jcb.org/cgi/content/full/jcb.200809090/DC1). At 37°C, the monopolar spindle was positioned distal to the cleavage furrow and seemingly adhered to the cortex at one side of the cell (Fig. 5 A and Video 1). The cytoplasts derived from this type of division contained scattered Golgi but no microtubules (Fig. 2, G and H; and Fig. 5, B and C). However, at a lower temperature, the spindle was positioned centrally in close proximity to the division plane (Fig. 5 E and Video 2), which allowed partial incorporation of spindle materials into the cytoplasts, as revealed by the presence of a microtubule network (Fig. 5 G). Furthermore, a Golgi ribbon reformed (n = 21; Fig. 5 F), suggesting that ribbon determinants were segregated into the cytoplasts. Therefore, these data support the idea that ribbon factors are bound to and partitioned together with the spindle.
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The cytoplasts received Golgi stacks capable of secretion independently of the spindle, but these stacks were not linked into a ribbon. This is in contrast to the karyoplasts, in which a ribbon reformed. Collectively, our data suggest two distinct mechanisms underlying Golgi inheritance. First, minimum functional Golgi units (stacks) are inherited in a spindle-independent manner. These stacks could be derived from Golgi that was partitioned together with the ER (Zaal et al., 1999) or could have reassembled from the Golgi that was segregated independently of the spindle (Jesch et al., 2001). Second, the mitotic spindle plays a vital role in transmitting ribbon determinants into the daughter cells.
The appearance of the Golgi ribbon in higher organisms during evolution reflects a different mechanism for polarized secretion. In lower animals such as Drosophila melanogaster, Golgi stacks are scattered and localized adjacent to ER exit sites despite the presence of centrosomes. Polarized secretion is achieved by targeting mRNA to specific ER exit sites where the cargo is made and secreted locally (Herpers and Rabouille, 2004). However, in mammalian cells, cargo is posttranslationally sorted from the centrally located Golgi ribbon (for review see Bard and Malhotra, 2006). To establish cell polarity, the entire Golgi ribbon is reoriented toward the site of secretion (Bisel et al., 2008), which is essential for a variety of cellular processes such as the outgrowth of dendrites in neurons (Horton et al., 2005), fibroblast migration during wound healing (Preisinger et al., 2004), and the immune response (Stinchcombe et al., 2006). Because the ribbon is particularly important for more advanced functions, tight coupling of ribbon determinants with the spindle ensures that each daughter cell receives the information to assemble it. This might be the reason that mammalian cells use the highly regulated spindle apparatus to partition these factors instead of a stochastic ER-dependent process.
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Materials and methods |
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TopAbstractIntroductionResults and discussionMaterials and methodsReferences |
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-tubulin (TAT1; provided by K. Gull, University of Oxford, Oxford, England, UK), FITC-conjugated -tubulin (DM1A; Sigma-Aldrich), dynein intermediate chains (74.1; Millipore), and nuclear pore complex (Mab414; Abcam). Rabbit polyclonal antibodies against GFP, S1P (Bartz et al., 2008), GRASP65 (provided by Y. Wang, University of Michigan, Ann Arbor, MI), p115 (provided by N. Nakamura, Kanazawa University, Kanazawa, Japan), pericentrin (Abcam), PDI (Assay Designs), Man I (provided by F. Barr, University of Liverpool, Liverpool, England, UK), Man II (provided by G. Warren, University of Vienna, Vienna, Austria), β-COP (EAGE; provided by R. Pepperkok, European Molecular Biology Laboratory, Heidelberg, Germany), p24
3 (provided by T. Nielsson, University of Gothenburg, Gothenburg, Sweden), syntaxin 5 (provided by A. Price, Yale University, New Haven, CT), Rab1, giantin (provided by M. Beard, Yale University, New Haven, CT), Rab6, and myc (Santa Cruz Biotechnology, Inc.) were used. Sheep polyclonal antibodies against rat serum albumin (provided by G. Warren) were used. Polyclonal antibodies were raised in rabbits against GST fusion proteins of mouse Golgin45 (residues 1–123), rat GRASP55 (residues 232–454), and rat GM130 (residues 1–73 [N73]). N73-specific antibodies were affinity purified using His-tagged N73 covalently attached to N-hydroxysuccinimide–activated Sepharose (GE Healthcare). Goat anti–rabbit and goat anti–mouse antibodies conjugated to Alexa Fluor 488, 555, 594, or 647 were obtained from Invitrogen, and HRP-conjugated secondary antibodies were obtained from Thermo Fisher Scientific.
Cell line, tissue culture conditions, and drug treatments
Rat kangaroo kidney cells (PtK1) stably expressing NAGT I–GFP (Jokitalo et al., 2001) were grown in medium A (F-12 medium, 100 U/ml penicillin, 100 µg/ml streptomycin, 2 mM glutamine (Invitrogen), and 10% cosmic calf serum [HyClone]) with 300 µg/ml G418 (EMD) at 37°C and 5% CO2. For live cell imaging, microinjections, immunofluorescence, and EM, PtK1 cells were grown on glass coverslips coated with Alcian blue 8GX (Sigma-Aldrich). To arrest cells in mitosis with monoasters, PtK1 cells were incubated for 2 h with an inhibitor of the kinesin Eg5, either 200 µM monastrol (BIOMOL International L.P.) or 20 µM S-trityl-l-cysteine (Acros Organics). To induce cell division, a Cdk1 inhibitor, either 50 µM roscovitine (EMD) or 25 µM purvalanol A (EMD), was added to medium. Microinjections of CD8 or myc–PDGF receptor mRNA and tubulin and/or Golgi extract were performed 2 h after addition of purvalanol A.
Protein purification and Golgi extraction
The oligomerization and Mad2-binding domain of Mad1 (residues 321–556; Canman et al., 2003) was cloned from IMAGE clone 4299982 (American Type Culture Collection) into pGEX4-T3 (GE Healthcare) purified on glutathione–Sepharose 4B (GE Healthcare), dialyzed against injection buffer (20 mM Hepes, pH 7.4, and 50 mM KOAc), and concentrated on a filter unit (Centricon YM-30; Millipore).
RLG membranes were purified as described previously (Wang et al., 2008). In brief, rat liver was homogenized in 0.5 M sucrose in PM buffer (potassium phosphate, pH 6.7, and 5 mM MgCl2) with protease inhibitor cocktail (Roche). The homogenate was layered on top of 0.86 M sucrose, overlaid with 0.25 M sucrose, and centrifuged for 60 min at 29,000 rpm in a rotor (SW-41; Beckman Coulter). The 0.5 M sucrose layer was collected (cytosol fraction). The interface between the 0.5 and 0.86 M sucrose (intermediate fraction) was diluted to 0.25 M sucrose and layered on top of 1.3 and 0.5 M sucrose. After centrifugation for 30 min at 8,000 rpm in a rotor (SW-41), the enriched RLG membranes were collected at the 0.5/1.3 M sucrose interface. For microinjection experiments, RLG membranes were pelleted by centrifugation at 13,000 rpm for 10 min at 4°C, washed three times with injection buffer, extracted for 15 min on ice with 10% n-octylglucoside (EMD), and centrifuged at 13,000 rpm for 10 min at 4°C. The pellet was solubilized in sample buffer (pellet fraction), and the supernatant was dialyzed (10-kD cut off) against injection buffer (supernatant fraction), centrifuged again, and concentrated on a filter unit (Centricon YM-10; Millipore). Tubulin purified from bovine brain was provided by M. Kikkawa (Kyoto University, Kyoto, Japan).
In vitro transcription of mRNA
The expression plasmid pDprotA was generated by subcloning the coding sequence of protein A into pDisplay (Invitrogen) between the signal sequence and the myc epitope followed by the transmembrane domain of the PDGF receptor. Linearized pCD8 (Wang et al., 2008) and pDprotA were transcribed in vitro using the mMESSAGE mMachine T7 Ultra kit (Applied Biosystems). Capping, poly(A)-tailing reactions, and recovery of the mRNAs by LiCl precipitation were performed according to the manufacturer's instructions.
Microinjection and live cell imaging
For time-lapse microscopy and microinjection experiments, cells were incubated in medium A containing 50 mM Hepes, pH 7.4. Microinjection was performed with a microinjector (Transjector 5246 or FemtoJet; Eppendorf) and a micromanipulator (5171; Eppendorf) connected to a microscope (Axiovert 200M; Carl Zeiss, Inc.; Bartz and Seemann, 2008). The reagents were injected at the following concentrations: 1.5 mg/ml Mad1 or Sar1dn (Bartz and Seemann, 2008), 0.2 mg/ml pCD8, 0.5 mg/ml CD8 or myc–PDGF receptor mRNA, 6 mg/ml tubulin, and 20 mg/ml Golgi extract. Mad1 was injected together with 2.5 mg/ml biotin-dextran as an injection marker and visualized by streptavidin–Alexa Fluor 350 (Invitrogen). All microinjection experiments were performed at least three times.
For time-lapse microscopy, coverslips were mounted into a chamber (Ludin; Life Imaging Services). The temperature was maintained using an incubator (XL-3; Carl Zeiss, Inc.) at 37°C unless otherwise stated. Phase-contrast images were taken at intervals of 3–20 min with an A-Plan 20x/0.3 PH1 objective (Carl Zeiss, Inc.) and a microscope (Axiovert 200M). Either a camera (Orca-285; Hamamatsu Photonics) and Openlab software (version 4.0.2; PerkinElmer) or a camera (DXM1200F; Nikon) in combination with MetaMorph software (version 7.1.3; MDS Analytical Technologies) was used.
Immunofluorescence and EM analysis
Cells were either fixed in 3.7% formaldehyde in PBS for 15 min and permeabilized in methanol at –20°C for 15 min or fixed and permeabilized in methanol at –20°C for 15 min and incubated with appropriate primary antibodies followed by secondary antibodies. DNA was stained with DRAQ5 (Biostatus) after RNase treatment or with Hoechst 33342 (Invitrogen). After staining, cells were mounted in Mowiol 4–88 (EMD). Upon the acquisition of time-lapse phase-contrast images, cells were fixed and stained in the chamber (Ludin) and repositioned onto the microscope stage to the original positions recorded during live cell imaging. Immunofluorescence analysis was performed with a Plan Neofluar 40x/1.3 differential interference contrast objective (Carl Zeiss, Inc.) and a camera (Orca-285) with the Openlab software (version 4.0.2). The contrast of the images was adjusted for the Golgi structures in the cytoplasts.
For quantitative analysis of the ribbon structure, the analyze particles function of ImageJ (National Institutes of Health) was used, and a fixed threshold was applied to all raw images (Puthenveedu et al., 2006). The Golgi was determined as a ribbon if 90% of the fluorescence intensity resided in no more than three continuous elements.
EM analysis was performed essentially as described previously (Wang et. al, 2008). Asymmetrical cell division was induced by treatment with trityl-cysteine (2 h) followed by purvalanol A (2 h) and monitored by video microscopy. Upon division, the cells surrounding the karyoplasts and cytoplasts were scraped off with a microinjection needle. The remaining cells were fixed in 2.5% glutaraldehyde in 0.1 M sodium cacodylate, pH 7.4, for 30 min, treated with 1% osmium tetroxide and 1.5% potassium cyanoferrate in 0.1 M cacodylate for 30 min, and embedded in Epon 812 (Electron Microscopy Sciences). Upon removal of the coverslips by hydrofluoric acid, thin sections were cut and stained with 2% uranyl acetate and lead citrate. Sections were analyzed on an electron microscope (Tecnai G2 Spirit; FEI Company), and images were captured on a charge-coupled device camera (USC1000 2k; Gatan). Stacks were defined as three or more cisternae separated by <20 nm.
Online supplemental material
Fig. S1 shows transport of newly synthesized proteins to the cell surface. Fig. S2 shows that temperature affects spindle positioning during division. Video 1 shows that PtK1 cells were induced to divide asymmetrically at 37°C. Video 2 shows that PtK1 cells were induced to divide asymmetrically at 32°C. Online supplemental material is available at http://www.jcb.org/cgi/content/full/jcb.200809090/DC1.
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Acknowledgments |
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J. Seemann is a Virginia Murchison Lithicum Scholar in Medical Research and is supported by a grant from the American Heart Association (8065090F).
Submitted: 12 September 2008
Accepted: 7 January 2009
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