Expression of a Wild-type CFTR Maintains the Integrity of the Biosynthetic/Secretory Pathway in Human Cystic Fibrosis Pancreatic Duct Cells
Laboratoire de Biologie Cellulaire et Moléculaire des Epithéliums, Université Paul Sabatier, France (EH,CS-C,LA,MF), and INSERM U531, Institut Louis Bugnard (IFR 31) CHU Rangueil, Toulouse Cedex, France (EH,MF)
Correspondence to: Prof. E. Hollande, Laboratoire de Biologie Cellulaire et Moléculaire des Epithéliums, Université Paul Sabatier, 38, rue des 36 Ponts, 31400 Toulouse, France. E-mail: hollande{at}cict.fr
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Summary |
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Key Words: cystic fibrosis Golgi complex microtubules protein trafficking carbonic anhydrase IV HCO3 secretion pancreas human
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Introduction |
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The Golgi complex plays an important role in the maturation, sorting, and transport of newly synthesized secreted lysosomal and plasma membrane proteins. In mammalian cells, this organelle is built up of stacks of flattened cisternae grouped together in the pericentrosomal region. Adjacent stacks are connected to each other by lateral tubules, forming a continuous ribbon-like structure (Rambourg and Clermont 1990). Each stack has a polarized structure and may be considered to be composed of at least three compartments: the cis-Golgi network (CGN)/cis-Golgi, the medial-Golgi cisternae, and the trans-Golgi/trans-Golgi network (TGN). The CGN/cis-Golgi, which receives newly synthesized proteins from the ERGIC, is where the first Golgi-specific glycosylation reactions occur. Each medial-Golgi cisterna contains specific enzymes that sequentially act to allow the addition or trimming of carbohydrate moieties. The trans-Golgi/TGN ensures the final glycosylation reactions and the sorting of proteins to the plasma membrane and lysosomes. The structural integrity of the Golgi complex is indispensable in the accurate sorting and transport of proteins to their final destination. Thus, during mitosis, the Golgi complex breaks down into small vesicles and the protein transport along the secretory pathway is arrested (Lowe et al. 1998
; Thyberg and Moskalewski 1998
). Various drugs, such as brefeldin A and okadaic acid, have a profound effect on the integrity of Golgi stacks, causing perturbations in protein maturation, sorting, and trafficking (Fujiwara et al. 1988
; Lucocq et al. 1991
; Tamaki and Yamashina 2002
). Microtubule-disrupting agents, such as nocodazole, also induce dispersal of Golgi stacks (Rogalski and Singer 1984
; Thyberg and Moskalewski 1985
; Cole et al. 1996
), often leading to a retardation in the transport of secreted and plasma membrane proteins (Matter et al. 1990
; Robin et al. 1995
; Cole et al. 1996
).
To determine whether the perturbations of CA IV traffic observed in CF cells result from changes in the Golgi complex, we analyzed the structure and distribution of this organelle with regard to the microtubule network in the pancreatic duct cell line CFPAC-1. We found a dispersal of Golgi stacks associated with disorganization of the microtubule cytoskeleton and an increase in the number of microtubule-organizing centers (MTOCs). Moreover, the reversion of CF cells by the wild-type CFTR led to the restoration of Golgi complex and microtubule distribution that allowed the correct trafficking of CA IV.
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Materials and Methods |
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Antibodies
Tight junctions were visualized using rabbit polyclonal antiserum against occludin from Zymed Laboratories (San Francisco, CA). To visualize membrane compartments, we used mouse monoclonal antibody against ERGIC-53 protein, kindly provided by Dr. Hans-Peter Hauri (Department of Pharmacology, Biocenter of the University Basel, Basel, Switzerland), mouse monoclonal antibody to 58K protein (clone 58K-9) from Sigma (St Louis, MO), and mouse monoclonal antibody to -adaptin (clone 88) from Transduction Laboratories (Lexington, KY). Anti-
-tubulin (clone DM1A) and anti-
-tubulin (clone GTU-88) monoclonal antibodies were purchased from Sigma. The rabbit polyclonal antiserum raised against the COOH terminal of human CA IV has been previously described (Fanjul et al. 2004
). FITC-labeled goat anti-rabbit IgG antibodies and TRICT-labeled goat anti-mouse IgG antibodies were from Nordic Laboratories (Tilburg, The Netherlands).
Cell Culture and Growth Assay
The CFPAC-1, CFPAC-PLJ-CFTR6, and CFPAC-PLJ6 cell lines were maintained in Iscove's modified Dulbecco's medium containing 10% fetal calf serum (Gibco BRL; Grand Island, NY), without antibiotics, except G418 (1 mg/ml) (Sigma) for the transfected lines (CFPAC-PLJ-CFTR6 and CFPAC-PLJ6). Cell cultures were maintained by successive passages using trypsin (0.05%)-EDTA (0.02%) (Gibco BRL) and were seeded at a concentration of 2 x 105 cells/ml in 25-cm2 flasks (Nunc; Roskilde, Denmark) and on glass coverslips coated with collagen I prepared from rat tail. Mycoplasma contamination was checked regularly using cultures in selective media and PCR (Mycoplasma PCR Primer Set; Stratagene, La Jolla, CA).
For growth assays, cells were seeded in Petri dishes at 1.7 x 105 cells/ml. Media was changed daily. Cell proliferation was measured every day (day 1 to day 7) by counting cells with a Malassez hemocytometer (Marienfeld Laboratory Glassware; Lauda-Koenigshofen, Germany). Mitotic index was estimated on 4-day-old cultures fixed with Bouin's solution (Sigma) and stained with hemalum-eosin. For each cell line, the mitotic index was calculated on three 1,000-cell samples from three separate experiments. The percentage of multipolar mitoses (number of multipolar mitoses/total number of cells) was also established.
Osmium Impregnation
Golgi complexes were visualized by light microscopy after osmium impregnation. Cells grown for 4 days were rinsed with phosphate buffered saline (PBS), then fixed in situ (24 hr; +4C) with Champy's mixture: osmium tetroxide (1%)-chromic acid (1%)-potassium dichromate (3%). After several rinses with distilled water, cells were treated with 1% osmium tetroxide for 7 days at +37C, then dehydrated and mounted with Depex mounting medium (EMS; Fort Washington, PA).
Transmission Electron Microscopy
To determine the ultrastructure of the Golgi complex, cells were fixed with glutaraldehyde (2.5%)-paraformaldehyde (2%) in cacodylate buffer (0.1 M; pH 7.2) for 1 hr at +4C, postfixed with 1% osmium tetroxide (45 min; +4C), dehydrated, and embedded in epon-araldite resin. Ultra-thin sections were stained with uranyl acetate and lead citrate, then observed in a Hitachi H600 electron microscope (Hitachi; Tokyo, Japan).
Staining with Fluorescent Dyes
Mitochondria were labeled using the MitoTracker Red CMXRos probe (Molecular Probes, Inc.; Eugene, OR). Briefly, 4-day-old cultures were incubated with 1 nM MitoTracker Red CMXRos in culture medium for 1 hr at 37C. Cells were then washed and fixed with paraformaldehyde (3%; 20 min). Samples were examined using a confocal laser microscope (LSM 410; Carl Zeiss, Iena, Germany) with helium laser excitation (543 nm).
Immunofluorescence
Immunofluorescence reactions were carried out on cells maintained for 46 days on glass coverslips coated with collagen I.
Tight Junctions
To check the polarized state of CFPAC-1, CFPAC-PLJ-CFTR6, and CFPAC-PLJ6 cells, tight junctions were revealed using antibody to occludin. Cells were fixed in a 95% methanol/5% acetic acid mixture for 10 min at 20C. After rinsing and blocking nonspecific antibody binding sites with 1% bovine serum albumin (BSA) in PBS, cells were incubated successively with polyclonal rabbit immune serum directed against occludin (1:50; 1 hr) in PBS:BSA followed by goat anti-rabbit IgG serum coupled with FITC (1:400; 45 min).
Golgi Compartments
CFPAC-1, CFPAC-PLJ-CFTR6, and mock cells were fixed in paraformaldehyde (3%; 20 min; +4C), then permeabilized in baths with increasing concentrations of alcohol. After rinsing and blocking of nonspecific antibody binding sites in PBS:BSA, cells were incubated overnight at +4C, either with the mouse monoclonal antibody to ERGIC-53 (1:800), the mouse monoclonal antibody to 58K protein (1:50), or the mouse monoclonal antibody to -adaptin (1:50), diluted in PBS:BSA. After rinsing, cells were incubated with TRITC-labeled goat anti-mouse IgG antibodies (1:100; 45 min). The distribution of Golgi compartments was also analyzed in cells treated with nocodazole, a microtubule-disrupting agent. Four-day-old cell cultures were treated for 2 hr with nocodazole (50 µM) dissolved in DMSO, or with DMSO (5 µl/ml) for controls. After rinsing, they were fixed, permeabilized, and processed for immunofluorescence staining with antibody to the 58K protein as described above.
CA IV
To detect CA IV in the various membrane compartments, double-labeling reactions of CA IV/ERGIC-53, CA IV/58K protein, and CA IV/-adaptin were performed. Briefly, cells were fixed in paraformaldehyde (PFA) (3%; 20 min), permeabilized in baths with increasing concentrations of alcohol, and then incubated, first with the rabbit polyclonal CA IV immune serum (1:100), then with mouse monoclonal antibody directed against ERGIC-53 (1:800), 58K protein (1:50) or
-adaptin (1:50). The antigenantibody complexes were revealed after incubation with anti-rabbit IgG coupled with FITC (1:200) and with anti-mouse IgG coupled with TRITC (1:100).
Microtubules
The microtubule cytoskeleton was visualized using antibody to -tubulin. Cells fixed in PFA (3%, 30 min) and permeabilized in baths with increasing concentrations of alcohol were incubated with mouse monoclonal anti-
-tubulin antibody (1:50). The antigenantibody complexes were revealed after incubation with anti-mouse IgG coupled with TRITC (1:100). Some reactions were also performed on cells previously treated with nocodazole to check for microtubule depolymerization.
MTOCs were detected using mouse monoclonal antibody to -tubulin (1:50) according to the method described above for the detection of
-tubulin.
Controls
The specificity of the immunocytochemical reactions was determined by incubating cells solely with the anti-rabbit IgG coupled with FITC or anti-mouse IgG coupled with TRITC.
Immunofluorescence samples were mounted in Fluorostab medium (ICN Biomedicals; Aurora, OH) and examined by confocal microscopy with an argon laser (488 nm) for FITC excitation and a helium laser (543 nm) for TRITC excitation. Serial optical sections were collected in the Z axis at 1-µm intervals.
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Results |
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Distribution of Golgi Complex
The different methods used to visualize the Golgi complex showed variations in its distribution and ultrastructure when compared in CFPAC-1 and CFPAC-PLJ-CFTR6 cells. In polarized CFPAC-1 cells, osmium impregnation revealed a large number of Golgi stacks dispersed throughout the cytoplasm (Figure 2a1). Each Golgi stack contained chromophilic (Figure 2a2, arrow) and chromophobic (Figure 2a2, arrowhead) regions corresponding to the cis and trans faces, respectively. They often appeared in groups of two or three (Figure 2a1, arrows). Electron microscopic examination confirmed this dispersed stack distribution. Figure 2b shows a polarized CFPAC-1 cell containing many small Golgi stacks disconnected from one another and scattered throughout the cytoplasm (Figure 2b, arrows). These stacks were unusual in that they were formed by dilated cisternae, often highly vesiculated (Figure 2c). In polarized CFPAC-PLJ-CFTR6 cells, Golgi stacks revealed by osmium impregnation were mostly grouped in the supranuclear cytoplasm (Figure 2d, arrows). Ultrastructural analysis showed a well-organized Golgi complex composed of large stacks with flattened cisternae (Figure 2e). Confocal microscopic examination of the immunocytochemical reactions using anti-58K protein antibodies demonstrated the presence of numerous Golgi stacks dispersed throughout the cytoplasm in polarized CFPAC-1 cells: (a) in focal planes passing through the bases of cells, few Golgi stacks were present (Figure 3a1); (b) in medial planes, a large number of stacks either isolated, or in small clusters (Figures 3a2 and 3a3, arrows) appeared throughout the cytoplasm; and (c) in supranuclear planes, there were very few or none at all (Figure 3a4). In polarized CFPAC-PLJ-CFTR6 cells, the distribution of Golgi stacks was different: they were absent in the basal cytoplasm (Figure 3b1), few in number in the medial cytoplasmic regions (Figure 3b2), and numerous and grouped in clusters in the supranuclear regions (Figures 3b3 and 3b4, arrows). We determined the number of cells presenting dispersed, partially dispersed, or clustered Golgi stacks using immunofluorescence images of different planes taken along the entire height of cells. For each cell line, we carried out counts of more than 200 cells per preparation (n=5). Statistical analyses of these data were performed using the non-parametric Mann-Whitney test. In the CFPAC-1 line, 90.1 ± 1.5% of the cells exhibited a dispersed and 4.1 ± 0.6% a clustered Golgi complex vs 12.4 ± 2.5% and 73.5 ± 4.1% in the CFPAC-PLJ-CFTR6 cell line (p<0.0001). A partially dispersed Golgi complex was observed in 5.7 ± 1.1% of CFPAC-1 cells and 14 ± 3% of CFPAC-PLJ-CFTR6 cells.
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Microtubules and the Golgi Complex
Confocal microscopic examination of -tubulin immunoreactivity showed differences in the distribution of microtubules between CFPAC-1 and CFPAC-PLJ-CFTR6 cells. In polarized CFPAC-1 cells, focal planes passing through the basal and medial cytoplasms displayed a network of dispersed microtubules that extended from the perinuclear regions to the periphery of cells (Figure 6a1). In polarized CFPAC-PLJ-CFTR6 cells, focal planes passing through the medial cytoplasms showed
-tubulin immunoreactivity located along lateral plasma membranes (Figure 6b1). In supranuclear cytoplasms of CFPAC-1 cells,
-tubulin immunoreactivity appeared as a network of dispersed filaments radiating from different focal points (Figure 6a2), whereas in CFPAC-PLJ-CFTR6 cells it appeared in the form of a dense, tangled, filamentous network (Figure 6b2). The addition of nocodazole to CFPAC-1 and CFPAC-PLJ-CFTR6 cell cultures resulted in complete microtubule depolymerization. The detection of the Golgi complex with anti-58K protein antibody revealed in CFPAC-1 cells treated with nocodazole a larger dispersal of Golgi elements (Figures 7a1 and 7a2) than in control cells, in which the Golgi elements often appeared in small clusters (Figures 7b1 and 7b2, arrows). The treatment of polarized CFPAC-PLJ-CFTR6 cells with nocodazole led to a dispersal of the Golgi complex (Figures 7c1 and 7c2) comparable to that obtained in treated CFPAC-1 cells. In untreated CFPAC-PLJ-CFTR6 cells, Golgi components were clustered in the supranuclear cytoplasm (Figures 7d1 and 7d2, arrows).
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Discussion |
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The human CF pancreatic duct cells of the CFPAC-1 line have been described as polarized cells (Schoumacher et al. 1990; Fanjul et al. 2002
) in which
F508 CFTR is not targeted to the plasma membrane (Demolombe et al. 1994
; Bannykh et al. 2000
; Fanjul et al. 2002
). In a recent study, we demonstrated perturbations in the intracellular trafficking of CA IV in CFPAC-1 cells (Fanjul et al. 2002
). CA IV is thought to play a role in the pancreatic HCO3 secretion (Mahieu et al. 1994
; Ishiguro et al. 1996
; Fanjul et al. 2004
), a mechanism impaired in CF (Kopelman et al. 1988
; Smith and Welsh 1992
; Lebenthal et al. 1993
; Choi et al. 2001
). CA IV is localized in the luminal membrane of normal human pancreatic duct cells (Fanjul et al. 2004
) and is trafficked via the Golgi complex (Mairal et al. 1996
). Generally, the intracellular trafficking of plasma membrane proteins involves spatial organization and continuity of rough endoplasmic reticulum, ERGIC, and Golgi compartments. In the first part of this work, we analyzed the integrity of the biosynthetic/secretory pathway in polarized CFPAC-1 cells and in the same cells transfected with the wild-type CFTR. Our different analyses demonstrated the dispersal of the Golgi complex associated with dilation and vesiculation of cisternae in CFPAC-1 cells. Structural changes of the Golgi complex have previously been described under various physiological, pathological, and experimental conditions. This is most notably the case in cells undergoing mitosis, in which Golgi stacks are broken down into tubulovesicular clusters (Lowe et al. 1998
; Thyberg and Moskalewski 1998
). In CFPAC-1 cells, the dispersal of Golgi elements does not concern exclusively cells undergoing mitosis, given that the mitotic index did not surpass 5%, whereas
90% of the cells displayed changes in Golgi complex distribution. Moreover, contrary to what occurs in mitotic cells, the integrity of Golgi stacks in CFPAC-1 cells was maintained, as demonstrated by electron microscopy. These structural changes with preservation of the Golgi stacks are similar to those described in human cells subjected to intracellular pH changes, such as those in colorectal cancer (Kellokumpu et al. 2002
) or hepatoma (Yoshida et al. 1999
). Further experiments are nevertheless necessary to establish whether disorganization of the Golgi complex in CF cellsin which changes in intracellular pH have been observed (Barasch et al. 1991
; Elgavish 1991
; Coakley et al. 2000
)are actually due to alterations in intracellular pH.
The structural integrity and positioning of the Golgi apparatus are dependent on the microtubule cytoskeleton (Thyberg and Moskalewski 1993,1999
; Marsh et al. 2001
). The distribution of Golgi stacks throughout the cytoplasm of CFPAC-1 cells could result from either a dysfunction in their attachment to microtubules or a change in microtubule distribution. With regard to the first possibility, the greater dispersal and fragmentation of Golgi elements observed in the CFPAC-1 cells treated with nocodazole is an argument in favor of their attachment to microtubules. However, this interpretation will require further experimental investigation. Regarding the second possibility, we demonstrated by immuncytochemistry an unusual distribution of the microtubule network in CFPAC-1 cells compared with reverted cells. Although in the reverted cells, microtubules extended from a supranuclear region corresponding to the centrosomal region and were also localized along the apico-basal axis, in
F508 CFPAC-1 cells, microtubules displayed a disorderly distribution and appeared to radiate from different focal points, distributed in a seemingly random fashion. This distinctive microtubule distribution suggested the existence of several nucleation sites. To test this hypothesis, we detected MTOCs using antibodies directed against
-tubulin. Although most cells in the reverted line contained one or two MTOCs, 63% of the CFPAC-1 cells exhibited an abnormally large number of MTOCs, suggesting the presence of supernumerary centrosomes. A multiplicity of centrosomes often appears in cancerous cells and is associated with multipolar mitoses (Sato et al. 2001
; Gisselsson et al. 2002
). In the present study, the number of multipolar mitoses in CFPAC-1 cells was not significantly different from that in the reverted cells and cannot, therefore, explain the abnormally elevated number of MTOCs. The causes of the multiplicity of MTOCs in CFPAC-1 cells and their nature, whether they are centrosomes or other types of MTOCs, like those described in polarized epithelial cells (Meads and Schroer 1995
), remain to be determined. A variety of data, however, suggesting that the Golgi complex plays a role in nucleation and the attachment of microtubules, could shed light on these two points (Chabin-Brion et al. 2001
). These authors demonstrated the association of a cytosolic fraction of
-tubulin with Golgi membranes and their capacity to nucleate microtubules. In CFPAC-1 cells, the numerous MTOCs could correspond to non-centrosomal nucleation sites of microtubules associated with Golgi stacks. In this case, the dispersal of the Golgi complex would be responsible for the large number of MTOCs and, consequently, the unusual distribution of the microtubule network.
The distinct distribution of mitochondria seen in CFPAC-1 cells compared with that in reverted cells may be related to disorganization of the microtubular cytoskeleton. It is known that microtubules are involved in mitochondrial distribution (Yaffe 1999) and, in addition, the fact that their distribution is similar to that of the Golgi complex in CFPAC-1 and CFPAC-PLJ-CFTR6 cells leads to the idea that they might be localized around the Golgi stacks. There, they would provide the energy needed for synthesis and secretion, as suggested recently by Dolman et al. (2005)
in the case of acinar cells.
The structural integrity of the Golgi complex is essential to its physiological functions with regard to maturation and transport of proteins. Perturbations in intracellular trafficking and sorting of proteins were observed in rat parotid acinar cells in which the structure of the Golgi complex was disrupted by brefeldin A and okadaic acid (Tamaki and Yamashina 2002). In a similar way, the fragmentation of the Golgi complex induced by microtubule-depolymerizing drugs is correlated with a drastic retardation in the transport of membrane and secreted proteins (Matter et al. 1990
; Robin et al. 1995
; Cole et al. 1996
). Furthermore, Graves et al. (2001)
demonstrated that expression of misfolded mutated growth hormone (mutation
32-71) causes fragmentation of the Golgi apparatus and interferes with the trafficking of other non-mutant proteins. In the case of CFPAC-1 cells, the disturbances in the intracellular trafficking of CA IV to the apical plasma membrane are probably due to disorganization of the Golgi complex. The presence of CA IV in ERGIC, Golgi cisternae, and TGN pointed to the ability of Golgi stacks to transfer this protein despite their scattering. On the other hand, their dispersal, associated with that of microtubules, probably perturbs the formation and trafficking of transport vesicles carrying CA IV from the TGN toward the apical plasma membrane. It is unlikely that CA IV would be the only protein whose trafficking is perturbed. Dispersal of Golgi components would lead to disruption of the transport of other membrane or secretory proteins in CF cells, as has already been documented for MRP8 and MRP14 (migration inhibitory factor-related proteins) in CFPAC-1 cells (Fanjul et al. 1995
). Perturbation of the secretory pathway could also explain why NHE3 expression is reduced in the luminal membrane of pancreatic duct cells from homozygote
F508 CFTR mice, as reported by Ahn et al. (2001)
. The fact that in reverted cells, both the Golgi complex and microtubules have a distribution consistent with that usually observed in polarized epithelial cells suggests the importance of CFTR in maintaining the integrity of the biosynthetic/secretory pathway. The molecular mechanism through which CFTR acts remains, nonetheless, to be determined.
Taken together, our results suggest that the disturbances in CA IV trafficking causing abnormalities in the pancreatic HCO3 secretion in CF could result from the disorganization of the microtubule network associated with the dispersal of the Golgi complex.
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Acknowledgments |
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We thank C. Baritaud for his technical assistance.
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Footnotes |
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Received for publication November 25, 2004; accepted May 11, 2005
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