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Article |
Correspondence to Paul D. Lampe: plampe{at}fhcrc.org
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Abstract |
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Abbreviations used in this paper: BIM, bisindolylmaleimide; CBX, carbenoxolone; Cx43, connexin43; Cx46, connexin46; Cx50, connexin50; HFK, human foreskin keratinocyte; pS368, phosphoserine368; S368, serine368.
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Introduction |
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Gap junctions are composed of integral membrane proteins called connexins. There are 20 connexin gene family members in humans, many of which have been cloned and characterized (Willecke et al., 2002; Saez et al., 2003). During intercellular channel formation, six connexin proteins oligomerize into a hexameric hemichannel, or connexon, that traffics to the plasma membrane. One hemichannel docks with a second, in an opposing cell, to form an intact channel. These channels can be gated in response to various stimuli, including changes in voltage, pH, and connexin phosphorylation (Saez et al., 2003).
Connexin43 (Cx43) is phosphorylated at multiple serine residues in a variety of cell types (Crow et al., 1990; Musil et al., 1990; Brissette et al., 1991; Laird et al., 1991; Berthoud et al., 1992). Phosphorylation of Cx43 can affect trafficking, assembly, degradation, and channel gating. After treatment with the PKC activator PMA, Cx43 phosphorylation is increased, and gap junctional communication is decreased, in several different cell types (Brissette et al., 1991; Berthoud et al., 1992, 1993; Reynhout et al., 1992; Lampe, 1994). Phosphorylation of Cx43 on serine368 (S368; phosphoserine368 [pS368]) increases upon PMA treatment and throughout the cell cycle, and results in a reduction in unitary channel conductance (50 picosiemens channels are favored over 100 picosiemens channels) (Lampe et al., 2000; Solan et al., 2003).
Expression of connexin genes is tissue specific and although several connexins can be found in skin, Cx43 is the predominant connexin in human epidermis and in cultures of human keratinocytes (Fitzgerald et al., 1994; Di et al., 2001). Keratinocyte proliferation occurs in the basal layer of the epidermis and keratinocytes undergo terminal differentiation as they migrate through the suprabasal and granular layers to the skin surface. Connexin proteins are differentially expressed in skin, with lower expression in the proliferative regions and higher expression upon differentiation (Risek et al., 1992; Goliger and Paul, 1994; Salomon et al., 1994; Lampe et al., 1998; Kretz et al., 2003).
Wounding of the epidermis activates cell migration across the wound bed, increases proliferation, and promotes changes in cell-to-cell communication (Clark, 1985; Grinnell, 1992; Gailit and Clark, 1994; Goliger and Paul, 1995; Martin, 1997; Kretz et al., 2003). It has been suggested that gap junctional intercellular communication may regulate certain aspects of the wound healing process, including initiation/synchronization of cellular migration (Goliger and Paul, 1995; Lampe et al., 1998; Kretz et al., 2003). After wounding, connexin expression is decreased at the wound edge but enhanced at unwounded adjacent areas and upon wound closure when the cells differentiate (Goliger and Paul, 1995; Saitoh et al., 1997; Lampe et al., 1998). Cx43 antisense application to wounds accelerated keratinocyte migration and the rate of wound repair, resulting in less scarring (Qiu et al., 2003). Closure of wounds was 1 d faster in Cx43-deficient mice (Kretz et al., 2003). These results indicate that Cx43 regulation plays an important role in wound repair.
We examined Cx43 phosphorylation on S368 in normal and wounded human skin tissue. In unwounded skin, basal keratinocytes, which show the lowest expression of total Cx43, showed similar levels of staining for pS368 to those shown by the suprabasal cells. Remarkably, 24 h after wounding, pS368 labeling was dramatically increased but strictly limited to the basal cells. The levels and distribution of pS368 returned to normal at 72 h. We "scratch wounded" primary human foreskin keratinocytes (HFKs) to test for changes in gap junctional communication and delineate the signaling pathways involved. Efficient migration to fill the scratch was dependent on gap junctional communication within the first 6 h. Scratch wounding increased phosphorylation on S368 at 24 h, and communication at the wound edge was reduced in a manner dependent on PKC. Thus, this report documents dynamic changes in Cx43 phosphorylation at a specific site that affects intercellular communication during the complex process of wound healing in HFKs and in human skin. The observation that basal cells near the wound edge show a temporally and spatially regulated change in their communication properties indicates that restriction of specific signals between epithelial cells occurs during wound healing.
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Results |
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Phosphorylation of Cx43 at S368 is limited to basal keratinocytes 24 h after wounding
Total Cx43 levels are diminished in the suprabasal cells near the wound edge after wounding (Goliger and Paul, 1995; Saitoh et al., 1997; Lampe et al., 1998). To determine the temporal regulation of S368 phosphorylation, we performed immunostaining on a time course of human wounds. We investigated Cx43 and pS368 levels in the wound bed region of wounds that had healed for 6 (Fig. 1, c and d), 24 (Fig. 1, e and f), and 72 h (Fig. 1, g and h). 6 h after wounding, little change in the normal distribution of Cx43 or pS368 antibody staining was observed, except a reduction in Cx43 levels that occurred in suprabasal cells within 50 µm of the wound (Fig. 1, c and d). At 24 h, an extensive reduction in suprabasal Cx43 staining and slight increases in basal cell levels occurred, yielding a more even distribution up to 300 µm from the wound bed (Fig. 1 e). In contrast, the levels of phosphorylation at S368 24 h after wounding were dramatically increased in basal keratinocytes and essentially absent throughout the rest of the epidermis (Fig. 1 f). This unique staining pattern extended up to 400 µm from the wound site, beyond which point pS368 and Cx43 levels normalized to the unwounded levels. In the magnified inset in Fig.1 f, the staining is present at interfaces between basal cells and at basal cellsuprabasal cell interfaces (shown without differential interference contrast optics or the line indicating the basement membrane). As a control, 24-h wounds were processed without the mouse or rabbit antibody, and little staining was observed when either was omitted from the staining procedure (Fig. 1 i, rabbit control shown). By 72 h after wounding, S368 phosphorylation expression patterns and levels were similar to those in unwounded skin. Thus, 24-h wounds showed a unique basal cell staining pattern for Cx43 phosphorylation at S368.
Cx43 phosphorylation on S368 in primary HFKs
Primary HFKs were used to allow examination of gap junctional communication and signaling pathways associated with the wounding process. To determine whether wounding of HFKs would affect phosphorylation at S368 consistent with in vivo wounds, we scratch wounded HFK monolayers with a pipette tip in a manner consistent with previous studies (e.g., Yamada et al., 2000). We performed immunofluorescence to determine whether changes elicited by scratch wounding paralleled those found in the in vivo wounds; i.e., whether pS368 levels increased near the scratch edge. Fig. 2 shows immunofluorescence of total Cx43 (A) and pS368 (B) in keratinocytes 24 h after scratch wounding. Although a reduction in Cx43 in the differentiating suprabasal cells was observed in wounds (Fig. 1 f), little change in Cx43 levels was observed near the scratch (Fig. 2 A), possibly because the cultured cells, like basal cells, are not differentiated. The ratio of pS368 to Cx43 signal, most clearly demonstrated in the overlay panel (Fig. 2 C), shows that the relative pS368 levels are highest 14 cell diameters from the scratch. Note that the signal for pS368 appears to be plasma membraneassociated and continuous throughout the cellcell interfaces, similar to the basal cell staining in the in situ wounds (Fig. 1 f, inset). The total Cx43 antibody used for this staining has a preference for the Cx43 present in gap junctions (Solan et al., 2003), so the continuous pS368 staining may represent protein that is not yet assembled into gap junctions. This possibility would be consistent with the observation that PKC activation inhibits the formation of new gap junctions (Lampe, 1994). Further away from the scratch, most of the pS368 signal overlays with the total Cx43 signal.
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Gap junctional communication was assayed by microinjection of Alexa Fluor 488 (with a molecular weight of 570.5) in keratinocytes present in 24-h scratch-wounded cultures, to determine whether phosphorylation at S368 affected the ability of HFKs to communicate. Examples of injections distant from and near the scratch edge and of the resulting dye transfer are shown in Fig. 4 A. In untreated cells (Fig. 4 B, CON), communication was limited to 4 cells when dye was injected near the scratch, compared with
25 cells in unwounded areas. When BIM was added to the scratch-wounded cells, gap junctional communication adjacent to the scratch occurred to
10 cells (Fig. 4 B) and was 2.4-fold more extensive (Fig. 4 C) than for the untreated cells injected at the scratch edge. Because cells injected adjacent to the scratch can only transfer away from the wound, the dye transfer levels would be expected to be less than half the level they are in cells that are injected internal to the wound. Thus, the BIM-treated cells adjacent to the scratch transferred dye nearly as efficiently as cells distant from the wound, whereas BIM had little apparent effect on the extent of dye transfer in cells injected far from the wound. Although Fig. 2 shows low levels of phosphorylation of Cx43 at S368 in cells distant from the scratch, apparently these levels are below a threshold level of phosphorylation necessary for detection of a reduction in gap junctional communication by dye transfer. Given the high specificity of BIM, these results indicate that PKC is likely integral to the wound signaling pathway responsible for the temporal reduction of communication of keratinocytes adjacent to human wounds.
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Discussion |
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Connexin proteins have distinct expression patterns in skin, with more expression upon differentiation (Risek et al., 1992; Goliger and Paul, 1994; Salomon et al., 1994). Similarly, the high level of S368 phosphorylation in basal cells near the wound delineates a communication compartment distinct from suprabasal cells. For example, signals produced by suprabasal cells that inhibit the initiation of migration or promote differentiation might not be passed to basal cells that are highly phosphorylated at S368. The highly specific temporal regulation is particularly noteworthy, as the only times these signals would be restricted are at 2448 h. Indeed, consistent with feedback control as observed in many signaling pathways, the levels of Cx43 and pS368 returned to the unwounded level after 72 h. Thus, in both the in situ wounds and scratch-wounded HFKs, phosphorylation at S368 appears to be a transient process that regulates communication in a time-dependent manner.
The purpose of Cx43 phosphorylation at S368 may also be to inhibit the ability of basal keratinocytes to communicate signals that initiate differentiation. Communication of different growth and differentiation signals by two related connexins has been shown in the lens, where connexin46 (Cx46) and connexin50 (Cx50) appear to transmit different signaling molecules (White, 2002). Knockout of either connexin results in cataracts, but lack of Cx50 also results in reduced ocular growth that is not relieved by knocking Cx46 into the Cx50 promoter. However, the knockin mouse no longer forms cataracts, indicating that Cx50 transmits different growth and differentiation signals from those transmitted by Cx46. Given the change in conductance properties associated with phosphorylation of Cx43 at S368, we believe that different differentiation/activation/migration signals may be transmitted by the basal keratinocytes as compared with the more differentiated layers, and that this regulation can be highly dynamic, as indicated by the wound studies.
During wound healing, epidermal cells must undergo changes in communication, proliferation, differentiation, migration, and activation (Clark, 1985; Grinnell, 1992; Gailit and Clark, 1994; Martin, 1997). Dynamic changes occur in the expression of specific proteins during wound repair. For example, wounding temporally alters expression of E-cadherin, laminin 5, p16, and integrin 6ß4 in basal keratinocytes at the wound edge (Stepp et al., 1996; Lampe et al., 1998; Natarajan et al., 2003). However, the timing and the highly specific compartmentalized localization of pS368 in basal cells distinctly point to specific migration/differentiation roles. Clearly, gap junctional communication that occurs before and after the 2448-h window would not be affected by S368 phosphorylation. Thus, early events such as increased production of laminin 5 and other activation events could still be signaled/regulated by gap junctional communication. Indeed, gap junctional communication before 6 h appears to be critical for migration, consistent with previous results indicating that cellular migration was inhibited in endothelial cells expressing dominant-negative Cx43 (Kwak et al., 2001) and that directionality of movement was reduced in Cx43-null neural crest cells (Xu et al., 2001). Furthermore, the reduction in gap junctional communication at 2448 h is a change in conductance, not a complete closure (Lampe et al., 2000). Therefore, the transfer of smaller, more permeable molecules will not be eliminated by this phosphorylation event. BIM treatment could then lead to temporally inappropriate transfer of larger, gap junctionpermeant molecules that might be important in regulating differentiation or coordination of migration. Alternatively, Cx43 phosphorylation might affect the interaction of Cx43 with proteins important in migration or differentiation. Consistent with these ideas, Xu et al. (2001) suggested that transfer of carboxyfluorescein, a relatively small dye with a molecular weight of 376.3, may not be a suitable gauge of the molecules important in neural crest cell motility, or Cx43-interacting proteins important in regulating motility might be affected by Cx43 conformational changespossibly caused by connexin phosphorylation. In any case, these results must be viewed with caution because dye transfer can be a poor predictor of the transfer of biologically important molecules (Goldberg et al., 2002) and BIM would be expected to have multiple effects on PKC-activated pathways that could influence migration and differentiation. For example, BIM pretreatment reduced keratinocyte migration by
30%, even though dye transfer increased. Thus, PKC-dependent pathways may enhance migration independent of Cx43.
A reduction in gap junctional communication several hours after wounding appears to be important in healing, as is evidenced by changes in connexin expression near the wound bed (Clark, 1985; Grinnell, 1992; Gailit and Clark, 1994; Goliger and Paul, 1995; Martin, 1997). Cx43 expression patterns and response to wounding differ in rodents and humans (Fitzgerald et al., 1994; Salomon et al., 1994; Goliger and Paul, 1995; Saitoh et al., 1997; Lampe et al., 1998; Richard, 2000; Di et al., 2001). However, the importance of tight regulation of gap junctional communication during the wounding process is evident. Wound closure occurred 1 d earlier (2 vs. 3 d) in Cx43-deficient mice, compared with wild-type controls (Kretz et al., 2003). Furthermore, Cx43 antisense application to wounds accelerated the rate of keratinocyte migration, reduced inflammation, and increased the rate of wound repair, resulting in less scarring (Qiu et al., 2003). Multiple signaling pathways regulate wound repair. Calcium levels play an important role in the regulation of wounded skin (Lansdown, 2002). Mitogen-activated protein kinases have been shown to coordinate migration and proliferation (Sharma et al., 2003). Many reports show that PKC plays a central regulatory role in wound repair, and PKC is activated by integrinextracellular matrix interactions after wounding (Clark and Brugge, 1995; Wallis et al., 2000). PKC can phosphorylate Cx43 at S368 (Fig. 3; Lampe et al., 2000), suggesting that PKC is a key component of the regulatory pathway that links the wounding event to changes in intercellular communication. The distinct distribution of pS368 in basal cells, the transient nature of the phosphorylation event, and the resulting change in gap junctional communication and migration all imply important roles for Cx43 in the regulation of epidermal cell activation after wounding and a role for gap junctions in forming a basal cellspecific "communication compartment" to spatially regulate these processes.
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Materials and methods |
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Immunostaining of tissues
6-µm cryostat sections of incisional wounds were immunolabeled using indirect immunoperoxidase, as described previously (Lampe et al., 1998). All tissue sections were postfixed in cold acetone and then labeled with primary antibodies mouse anti-Cx43 (Cx43NTI; described in Goldberg et al., 2002; Solan et al., 2003) or anti-phosphoconnexin 43 Ser368 (Cell Signaling Technology) at dilutions of 1:1,200 and 1:250, respectively. We detected signal using biotinylated goat antirabbit and biotinylated horse antimouse (Vector Laboratories) at dilutions of 1:400 and 1:200, respectively, with a streptavidin complex kit (SABC; Vector Laboratories), 0.12% 3, 3' diaminobenzidine for the chromogen, and Glycergel (DakoCytomation) as mounting media. All tissue images were viewed with a microscope (Microphot-SA; Nikon), using brightfield and differential interference contrast optics.
Cells and cell culture
Normal primary HFKs were prepared as described previously (Boyce and Ham, 1983). Cells were maintained in serum-free keratinocyte growth medium (Clonetics Corp.) containing insulin, epidermal growth factor, hydrocortisone, and bovine pituitary extract in a humidified 5% CO2 incubator at 37°C. To mimic wounding, parallel 9095% confluent HFK cultures grown on 60-mm culture dishes were left untreated or were scratch wounded with a plastic pipette tip. Immunofluorescence was performed as described previously (Brown et al., 2004), using formaldehyde fixation and Alexa Fluor 488labeled goat antirabbit and Alexa Fluor 594 goat antimouse (both highly cross-adsorbed; Molecular Probes), on a scanning confocal microscope (Meta Multi-Photon, LSM 510; Carl Zeiss MicroImaging, Inc.) using Argon (488 nm) and HeNe (543 nm) lasers with a 40x/1.3 oil objective (Plan Neofluar). For immunoblot analysis, cultures were consistently "scratched" in a spiral pattern followed by a crosshatch pattern in the absence (control) or presence of the kinase inhibitors PD98059, Gö6983, chelerythrine, K252a, BIM, and Ro-31-8220 (all from Calbiochem). Cells were washed once with PBS and harvested on ice-cold 1% Triton X-100 in PBS or 2% SDS sample buffer, both containing 500 µM Na3VO4, 50 mM NaF, 2 mM PMSF, and 1x Complete protease inhibitors (Roche Diagnostics), as performed previously (Solan et al., 2003).
Immunoblot detection of Cx43 and pS368 levels
Cellular proteins were separated by SDS-PAGE (10% acrylamide). Proteins were transferred to nitrocellulose, the membrane was blocked in 1% milk in PBS, and Cx43 and pS368 were detected simultaneously on the same blot using mouse anti-Cx43 (Cx43NT1) at a dilution of 1:5,000 and rabbit anti-phosphoCx43 S368 at a dilution of 1:1,000, in blocking solution. Membranes were washed three times with PBS for 15 min per wash, and primary antibodies were detected using IRDye800donkey antimouse (Rockland) and goat antirabbit Alexa Fluor 680 (Molecular Probes) secondary antibodies diluted at 1:2,500. The absolute levels of these antibodies were directly detected by fluorescence using the Odyssey image analysis system (LI-COR Biotechnology). To determine the ratio of Cx43 to pS368, fluorescence values were ratioed and then divided by the zero time for the time course experiment or the control value for the drug treatment experiment to yield the relative ratio for each time point. The relative ratios were averaged across experiments and the SEM was calculated for each time point.
In vitro phosphorylation and detection of pS368 were performed with the COOH-terminal portion (amino acids 246382) of Cx43 containing six NH2-terminal histidine residues (Cooper and Lampe, 2002) and purified PKC (Panvera), according to previously published methods (Lampe et al., 2000).
Microinjection and migration studies
HFKs were grown on 60-mm dishes to confluency and, where indicated (Fig. 4), were either scratch wounded as described above or left unwounded, in the presence or absence of 200 nM BIM. Injections were performed on an inverted microscope (Diaphot, model TE300; Nikon) with phase and fluorescence optics, using a micromanipulator (Narashigi). Micropipettes were drawn from borosilicate glass capillaries (Kwik-Fil; World Precision Instruments, Inc.; 1.0-mm OD x 0.75 mm). 10 mM Alexa Fluor 488 (570.5 Mr) in 0.2 M KCl was injected until the injected cell was brightly fluorescent, and then the pipette was removed. The number of cells receiving dye when coupled (i.e., the extent of dye coupling) was assessed 3 min after microinjection with a cooled digital camera (MicroMax; Princeton Instruments) driven by an attached PC and Metamorph imaging software. For migration studies, HFKs were grown on 100-mm dishes and scratch wounded with a cell lifter along marked lines. Specific areas for measurement were also marked, and digital images were taken with the inverted microscope (Nikon) immediately after scraping and at 6, 24, and 48 h. Where indicated (Fig. 5), 15 µM CBX (3-hydroxy-11-oxoolean-12-en-30-oicacid 3-hemisuccinate) or 200 nM BIM was added. After alignment, images were superimposed and migration distances were measured. Three random positions per image were measured and at least 20 images were collected per experiment. Results from three separate experiments were compiled by taking the ratio of the distance migrated at 6 and 24 h relative to the distance the untreated cells migrated at 48 h. Standard error was calculated and results were compared with a two-tailed, unequal variance t test. For measurement of migration front regularity, the length of a line drawn along the front edge of the leading cells after 48 h of migration was measured relative to the length of a line drawn immediately after the scratch was performed. These measurements were compared between BIM-treated and untreated cultures using a two-tailed, unequal variance t test.
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Acknowledgments |
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Submitted: 23 April 2004
Accepted: 16 September 2004
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References |
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