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ERK regulates Golgi and centrosome orientation towards the leading edge through GRASP65
Correspondence to Joachim Seemann: joachim.seemann{at}utsouthwestern.edu
Directed cell migration requires the orientation of the Golgi and centrosome toward the leading edge. We show that stimulation of interphase cells with the mitogens epidermal growth factor or lysophosphatidic acid activates the extracellular signal–regulated kinase (ERK), which phosphorylates the Golgi structural protein GRASP65 at serine 277. Expression of a GRASP65 Ser277 to alanine mutant or a GRASP65 1–201 truncation mutant, neither of which can be phosphorylated by ERK, prevents Golgi orientation to the leading edge in a wound assay. We show that phosphorylation of GRASP65 with recombinant ERK leads to the loss of GRASP65 oligomerization and causes Golgi cisternal unstacking. Furthermore, preventing Golgi polarization by expressing mutated GRASP65 inhibits centrosome orientation, which is rescued upon disassembly of the Golgi structure by brefeldin A. We conclude that Golgi remodeling, mediated by phosphorylation of GRASP65 by ERK, is critical for the establishment of cell polarity in migrating cells.
S.-i. Yoshimura's present address is University of Liverpool, Cancer Research Centre, Liverpool L3 9TA, England, UK.
Abbreviations used in this paper: BFA, brefeldin A; ERK, extracellular signal–regulated kinase; LPA, lysophosphatidic acid; MEK, MAPK/ERK kinase; NRK, normal rat kidney; RLG, rat liver Golgi.
© 2008 Bisel et al. This article is distributed under the terms of an Attribution–Noncommercial–Share Alike–No Mirror Sites license for the first six months after the publication date (see http://www.jcb.org/misc/terms.shtml). After six months it is available under a Creative Commons License (Attribution–Noncommercial–Share Alike 3.0 Unported license, as described at http://creativecommons.org/licenses/by-nc-sa/3.0/).
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Introduction |
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Several lines of evidence suggest important roles for the polarized localization of the Golgi at the leading edge. Cell migration requires the regulated transport of vesicles and the addition of new membranes to the leading edge (Jaffe and Hall, 2005). Polarized secretion at the leading edge is regulated by the exocyst, which is essential for exocytosis, and also organizes actin polarization at the leading edge (Zuo et al., 2006). In addition, the directional delivery of membranes and proteins toward the leading edge is dependent on Golgi-localized protein kinase D, which regulates the formation of transport vesicles from the trans-Golgi network to the plasma membrane (Liljedahl et al., 2001). Inhibition of protein kinase D blocks both membrane delivery to the cell surface and directional cell migration (Prigozhina and Waterman-Storer, 2004). These examples suggest that vesicle formation and fusion are tightly coupled to directed cell motility. Additionally, delivery of adhesion molecules and cytoskeletal components are all important functions of a polarized Golgi (Mellor, 2004).
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Results and discussion |
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To test whether ERK modifies the regulatory domain of GRASP65 during Golgi polarization, we expressed the GRASP domain (residues 1–201) fused to GFP (Fig. 1 C). Because GRASP65 1–201 is insensitive to kinase activity, a constitutive oligomer, and prevents cisternae from unstacking or remodeling, the mutant should delay or inhibit Golgi orientation. After expression of the cDNA in wound-edge cells by microinjection, we assessed Golgi orientation in response to mitogens. Fig. 1 D shows a typical immunofluorescence image of cells at the wound edge expressing either GRASP65 1–201 or the control protein G2A GRASP65 1–201, where the glycine at position two is replaced by an alanine (G2A) to abolish the myristoylation, and therefore Golgi targeting (Fig. 1 C; Barr et al., 1998). In control cells and cells expressing G2A GRASP65 1–202, the Golgi achieve maximum orientation after 90-min stimulation with LPA, whereas in cells expressing GRASP65 1–202, inhibition of Golgi orientation is observed after 90 min and maintained after a 270-min addition of LPA (Fig. 1 E). The inhibitory effect of GRASP65 1–201 on Golgi polarization persisted after stimulation with serum, EGF, or LPA for 90 min (Fig. 1 F), suggesting that the regulatory domain of GRASP65 is essential for mitogen-stimulated Golgi orientation.
GRASP65 is phosphorylated at Ser277 by ERK (Yoshimura et al., 2005). GRASP65 is also phosphorylated in mitosis at Ser277 and at three other sites by cdk1/cyclinB1 (Preisinger et al., 2005). To test if GRASP65 phosphorylation by ERK is induced by other mitogens known to cause Golgi orientation, we used a previously characterized antibody against phospho-Ser277 of GRASP65, which also recognizes mitotically phosphorylated GRASP65 (Yoshimura et al., 2005). In the absence of mitogens, the phospho-GRASP65 antibody stained mitotic cells (Fig. 2 A), whereas the surrounding interphase cells showed little or no signal (images acquired equally). Stimulation with serum, EGF, or LPA considerably increased phosphorylation of GRASP65 in interphase cells (Fig. 2 B). U0126 abolished GRASP65 phosphorylation in interphase cells, whereas the mitotic signal was unaffected (Fig. 2, A and B), suggesting separate regulation of GRASP65 phosphorylation in mitosis and interphase (Yoshimura et al., 2005).
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During cell migration, the centrosome orients toward the leading edge, as does the Golgi (Magdalena et al., 2003; Cau and Hall, 2005). Thus, we explored whether centrosome orientation is linked to Golgi orientation using the GRASP65 mutants that inhibit Golgi polarization (Fig. 5 A). In cells expressing S277A GRASP65 FL or GRASP65 1–201, centrosome orientation was significantly inhibited, whereas centrosomes of control protein or nonexpressing cells oriented as expected (Fig. 5, B and C), consistent with our quantitation of Golgi polarization (Fig. 1 E and Fig. 3). The fact that centrosomes always localized with the Golgi suggests that tight coupling between these two organelles is preserved during cell polarization.
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We have explored the effects of ERK phosphorylation on GRASP65 during Golgi orientation toward the direction of cell migration. Our data indicate that ERK phosphorylates GRASP65 in interphase cells, resulting in the loss of GRASP65 oligomerization and causing subsequent Golgi cisternal unstacking. Preventing GRASP65 phosphorylation with phosphorylation-resistant mutants inhibits Golgi and centrosome orientation, leading to the conclusion that Golgi remodeling by kinase signaling is critical for the polarization of migrating cells.
Golgi remodeling has been best described in mitosis, where unstacking and vesiculation are driven by the phosphorylation of Golgi proteins including GM130, GRASP65, and GRASP55 (Shorter and Warren, 2002). Phosphorylation of GRASP65 by mitotic kinases leads to the loss of oligomerization followed by unstacking and lateral unlinking of Golgi cisternae (Barr et al., 1997; Wang et al., 2003; Feinstein and Linstedt, 2007). Ser277 of GRASP65 is phosphorylated in mitosis by cdk1/cyclinB1 and by ERK in interphase (Yoshimura et al., 2005), suggesting that GRASP65 phosphorylation may organize similar processes during interphase and mitosis. We report here that inhibiting interphase GRASP65 phosphorylation by ERK prevents Golgi reorganization, which is required for Golgi polarization. We conclude that interphase and mitotic phosphorylation of GRASP65, although differently regulated and required for unique cellular processes, produce similar consequences for Golgi structure, including loss of oligomerization and unstacking of cisternae. Therefore, phosphorylation of GRASP65 functions to regulate Golgi remodeling whether during mitosis or cell polarization.
The fragmented Golgi structure of mitotic cells is, however, not found during interphase by light microscopy (Yoshimura et al., 2005). The amount of Golgi reorganization could be a function of the extent of GRASP65 phosphorylation. GRASP65 phosphorylation in mitosis involves at least four distinct sites (Preisinger et al., 2005), but only Ser277 is known to be phosphorylated during interphase (Yoshimura et al., 2005). Additionally, mitotic Golgi fragmentation depends on the phosphorylation of other Golgi proteins, including GM130 and GRASP55, which are not phosphorylated during interphase (Lowe et al., 1998; Feinstein and Linstedt, 2007). Therefore, decreased GRASP65 phosphorylation and the lack of phosphorylation of other Golgi proteins correlate to the lesser extent of Golgi remodeling during interphase. Maintaining the Golgi structure and organization in polarizing cells would allow for the quick upstart of directed membrane traffic necessary for migration once the Golgi faces the leading edge.
In summary, our work reveals that remodeling of the Golgi structure is required for the polarization of the Golgi toward the direction of cell migration. The Golgi remodeling is achieved by phosphorylation of GRASP65 by ERK, causing loss of GRASP65 oligomerization and cisternal unstacking. Furthermore, we found that centrosome polarization cannot be achieved without Golgi remodeling, showing that Golgi remodeling is critical for cell polarization.
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Materials and methods |
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-tubulin (GTU-88; Sigma-Aldrich), and GRASP65 (F. Barr, University of Liverpool, Liverpool, UK) were used. Hoechst 33342 and secondary antibodies conjugated to Alexa Fluor 488, 555, 594, or 643 were purchased from Invitrogen, and HRP-conjugated secondary antibodies were purchased from Thermo Fisher Scientific.
Cell culture and wounding
NRK cells were maintained in medium A (DME 100 U/ml penicillin, 100 µg/ml streptomycin, and 2 mM glutamate [Invitrogen]) with 10% cosmic calf serum (HyClone) at 37°C and 5% CO2. Cells were grown on glass coverslips until confluency and starved for 24 h in medium A without serum before Western blot analysis or wounding. Wound edges were created with a razor blade and the cells were allowed to recover for 2 h before microinjection. For experiments not involving microinjection, cells were wounded 5 h before addition of serum to be consistent with microinjection experiments. To inhibit ERK activation, 10 µM U0126 was added 30 min before stimulation with 1% serum.
To detect GRASP65 phosphorylation, serum-starved NRK cells were treated for 10 min with 0.1% serum, 2 ng/ml EGF, or 2 µM LPA. To inhibit ERK activation, the cells were preincubated for 30 min with 20 µM U0126. The cells were then analyzed by immunofluorescence or lysed for 15 min on ice in TEGN buffer (10 mM Tris-HCl, pH 7.4, 420 mM NaCl, 10% glycerol, 0.5% NP-40, and 1 mM EDTA), 1 mM DTT, 1 mM PMSF, 10 mM β-glycerophosphate, 10 mM NaF, and protease inhibitor cocktail (Roche). The extracts were cleared by centrifugation for 15 min at 15,000 g and subjected to 10% SDS-PAGE followed by Western blotting analysis.
Microinjection
The following constructs were used: pEGFP 1–201 GRASP65, pEGFP G2A GRASP65 1–201 (Wang et al., 2005), pcDNA3.1 GRASP65, and pcDNA3.1 S277A GRASP65 (Yoshimura et al., 2005). Cells in Hepes medium (DME, 25 mM Hepes, and no calf serum) were microinjected as described previously (Bartz and Seemann, 2008) with 0.1 mg/ml plasmid and incubated at 37°C for 2 h to allow protein expression. 2 µM LPA (bound to fatty-acid free BSA), 2 ng/ml EGF, or 0.1% serum was added to induce cell polarization.
Immunofluorescence and image analysis
Cells were fixed and permeabilized for 10 min in methanol at –20°C and incubated with the indicated antibodies followed by fluorescent secondary antibodies. DNA was stained with Hoechst 33342. Fluorescence analysis was performed with a 40x/1.4 differential interference contrast objective (Plan-Apochromat; Carl Zeiss, Inc.) and a microscope (Axiovert 200 M; Carl Zeiss, Inc.). Images were captured with a camera (Orca-285; Hamamatsu Photonics) and the software package Openlab (4.02; Improvision).
Quantitation of Golgi and centrosome polarization
The Golgi was stained for GM130 and centrosomes for -tubulin. Golgi and centrosome orientation was determined for the first row of cells facing the wound as described previously (Etienne-Manneville and Hall, 2001; Gomes et al., 2005) and counted as oriented if the majority was located in a 120° sector emerging from the center of the nucleus and facing the wound edge. Basal levels of expected random orientation of 33% are marked by red lines in the graphs. Percentage of Golgi or centrosome orientation was calculated by dividing the number of oriented cells by the number of total cells for each condition. The mean percentage from three or more experiments were averaged and presented as a mean ± SEM. Statistical analysis was performed using Student's t tests and significance was assigned for P < 0.05. P-values compared with each of the control conditions are represented by asterisks.
Golgi unstacking assay
120 µg of RLG membranes (Wang et al., 2003), with or without pretreatment for 30 min with 20 µM U0126 or 10 µM staurosporine, were incubated with 6 µg of recombinant purified MEK1 and ERK2 in 0.4 ml MEB buffer (50 mM Tris-HCl, pH 7.3, 50 mM KCl, 10 mM MgCl2, 15 mM EGTA, 20 mM β-glycerophosphate, 0.2 M sucrose, 2 mM ATP, 1 mM GTP, and 1 mM glutathione) for 20 min at 37°C. The reactions were then subjected to 10% SDS-PAGE and analyzed by Western blotting. For EM analysis, the reactions were fixed with 2% glutaraldehyde and processed as described previously (Wang et al., 2003). The relative proportion of stacked and unstacked membranes was determined by the intersection method (Wang et al., 2003).
Bead aggregation assay
Phosphorylation-dependent oligomerization of GRASP65 was determined as described previously (Wang et al., 2003). Recombinant GRASP65 FL and S277A mutant were purified as described previously (Wang et al., 2005), cleared by centrifugation at 15,000 g for 30 min, and cross-linked to M500 beads (Invitrogen). The beads were incubated for 60 min at 37°C with interphase HeLa cytosol (Wang et al., 2003) in KHM buffer (25 mM Hepes, pH 7.3, 60 mM KCl, 5 mM Mg(OAc)2, 0.2 M sucrose, and 1 mM glutathione) to allow aggregation. The beads were washed with MEB buffer, incubated for 60 min at 37°C with MEK1 and ERK2 in MEB buffer, and observed by phase-contrast microscopy. The percentage of beads in aggregates was quantified as described previously (Wang et al., 2003).
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Acknowledgments |
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Y. Wang is supported by the Pardee Cancer Research Foundation. J. Seemann is a Virginia Murchison Lithicum Scholar in Medical Research. This work was supported by a grant from the American Cancer Society to J. Seemann (ACS-IRG-02-196).
Submitted: 9 May 2008
Accepted: 31 July 2008
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3 independent experiments for each condition or time point. *, P < 0.05; ***, P < 0.001.
