* Toxicology Program, Department of Environmental Health, University of Michigan, 1420 Washington Heights, Ann Arbor, Michigan 48109-2029; National Food Safety & Toxicology Center and Department of Pediatrics and Human Development, Michigan State University, 243 Food Safety, East Lansing, Michigan 48824-1302; and
National Food Safety & Toxicology Center and Department of Pediatrics and Human Development, Michigan State University, 246 Food Safety, East Lansing, Michigan 48824-1302
1 To whom correspondence should be addressed. Fax: (734) 647-9770. E-mail: rlc{at}umich.edu.
Received February 24, 2005; accepted May 13, 2005
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ABSTRACT |
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Key Words: glutathione; lindane; -hexachlorocyclohexane; gap junctions; myometrium; oxidative stress.
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INTRODUCTION |
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Lindane, -hexachlorocyclohexane, is a pesticide that bioaccumulates in human adipose tissue (Robinson et al., 1990
). Lindane-induced inhibition of gap junction communication was first observed in Chinese hamster fibroblasts (Tsushimoto et al., 1983
) and more recently reported in myometrial myocytes (Criswell and Loch-Caruso, 1995
; Criswell et al., 1995
). Lindane inhibits gap junction intercellular communication between rat myometrial cells in a biphasic, temporal manner, characterized by an initial acute inhibition in the presence of lindane followed by rapid reversal after termination of lindane exposure, and then the subsequent redevelopment of a secondary, delayed-onset inhibition of gap junction intercellular communication without further exposure (Krieger and Loch-Caruso, 2001
; Loch-Caruso et al., 2003
).
Lindane inhibits gap junction intercellular communication by a mechanism that involves oxidative stress, as shown in hepatocytes (Ruch and Klaunig, 1986) and myometrial cells (Krieger and Loch-Caruso, 2001
). Oxidative stress occurs when the redox state of the cell is perturbed with either an overproduction or underproduction of oxidants that can damage the macromolecular machinery of the cell or perturb cell signaling. Glutathione (L-
-glutamyl-L-cysteinylglycine) is a predominant low molecular weight cellular thiol that is important for various cellular processes, including protection against damage from reactive oxygen species and free radicals that arise during conditions of oxidative stress (Meister and Anderson, 1983
).
Glutathione is formed intracellularly in its reduced state. Reduced glutathione (GSH) is essential for the formation of DNA precursors, amino acid transport, and reduction of disulfide linkages, among other functions. The sulfhydryl moiety of GSH is particularly reactive and can serve as a nucleophile, reductant, and free radical scavenger. Reactions involving GSH as a reductant normally lead to GSH oxidation to a disulfide form, GSSG (Mannervik et al., 1989), and decreased GSH/GSSG ratios that are associated with oxidative stress (Gardiner and Reed, 1994
). Consistent with lindane's pro-oxidant activity, lindane depressed cellular GSH in rat liver (Barros et al., 1988
; Videla et al., 1990
) and in rat embryos and visceral yolk sac (McNutt and Harris, 1994
). Although earlier reports indicate that lindane induces oxidative stress in myometrial cells (Krieger and Loch-Caruso, 2001
), effects of lindane on GSH and GSSG in myometrial cells have not been reported previously. The current study evaluates the hypothesis that oxidation of GSH to GSSG is a component of the mechanism by which lindane inhibits myometrial gap junction intercellular communication.
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MATERIALS AND METHODS |
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Cell isolation and culture.
Myometrial smooth muscle cells were isolated from midgestation (Day 10) Sprague-Dawley rats as previously described (Loch-Caruso et al., 1992). Myometrial cells established by this procedure express the gap junction protein connexin43 and regulate gap junctions in a manner consistent with in vivo responses (Caruso et al., 1990
; Loch-Caruso, 1999
; Loch-Caruso et al., 1992
). Briefly, rats were anesthetized with ether and euthanized by exsanguination or cardiac puncture. Uteri were removed to ice-cold physiologic saline solution (PSS) containing 135 mM NaCl, 5 mM KCl, 1.2 mM MgCl2, 1 mM CaCl2, 1 mM Hepes, and 5 mM glucose, adjusted to pH 7.4 with 1 N NaOH. Each uterus was dissected free of embryos, cervix, ovaries, and adipose tissue, then diced and digested in an enzyme solution containing 300 µg/ml type II collagenase, 300 µg/ml type III trypsin, and 200 µg/ml deoxyribonuclease I. The digest was filtered to remove large tissue clumps and the filtrate was centrifuged to pellet the cells. After repeated washing of the cells with calcium/magnesium-free phosphate-buffered saline (CMF-PBS; 2.68 mM KCl, 1.5 mM K3PO4 [monobasic], 136.9 mM NaCl, 8.1 mM Na3PO4 [dibasic heptahydrate] at pH 7.2), cells were seeded into flasks containing RPMI medium supplemented with 10% BCS. Cells were incubated at 37°C with 5% CO2 atmospheric conditions. The medium was changed every two days, and cells were subcultured every 67 days just before confluence. Isolated cells were characterized as smooth muscle cells by indirect immunofluorescence labeling with mouse anti-
-smooth muscle-specific actin monoclonal antibody as described previously (Caruso et al., 1990
). Alpha-actin labeling indicated cultures were at least 99% smooth muscle cells. Unless otherwise indicated, all experiments used myometrial cells at passage two and all incubations were at 37°C in a 5% CO2/95% air atmosphere using RPMI medium supplemented with 10% BCS.
Lindane exposure.
Cells were incubated for 1 h in RPMI medium containing 100 µM lindane derived from a stock solution of 50 mM lindane in dimethyl sulfoxide (DMSO). For the dye transfer experiments, cell cultures were either immediately processed for microinjection with Lucifer yellow dye or were rinsed three times with pre-warmed CMF-PBS after the 1-h lindane exposure, and then incubated with fresh medium without lindane for 0.25, 0.5, 1, 4, 24, 48, or 96 h before microinjection with Lucifer yellow dye. A minimum of 10 cells per culture dish were microinjected with Lucifer yellow dye and there were 67 dishes per treatment group. Myometrial cells were treated in a similar manner for HPLC evaluation of cellular GSH and GSSG immediately after a 1-h exposure to 100 µM lindane or 0.5, 1, or 24 h after 1-h exposure to 100 µM lindane (four culture dishes per treatment group). Solvent controls were incubated for 1 h in medium containing 0.2% DMSO and treated in a manner identical to the cultures exposed to lindane.
Diamide exposure.
To promote oxidation of GSH to GSSG, myometrial cells were exposed to 50 µM diamide for 0.5 h. Solvent controls were exposed to 0.05% double distilled water (DDW). At the end of the exposure, the cells were microinjected and assessed for Lucifer yellow dye transfer in diamide-containing medium. The concentration and exposure duration for diamide were based on experiments in our laboratory that showed a maximal inhibitory effect on Lucifer yellow dye transfer under these conditions (data not shown). A minimum of six cells were microinjected in each of five dishes per treatment group.
Exposure to 1,3-bis(2-chloroethyl)-1-nitrosourea (BCNU).
Cells were exposed to the GSSG reductase inhibitor 1,3-bis(2-chloroethyl)-1-nitrosourea (BCNU) to prevent reduction of GSSG to GSH. Cells in culture were exposed for 4 h to 25 µM BCNU or to 0.05% DMSO (solvent control). At the end of the exposure time, the cells were microinjected and assessed for Lucifer yellow dye transfer in BCNU-containing medium. Exposure to 25 µM BCNU for 3 h produced virtually identical results as the exposure for 4 h (data not shown). A minimum of six cells were microinjected in each of five dishes per treatment group.
Lucifer yellow dye transfer.
To assess gap junction intercellular communication, myometrial cells in culture were injected with mixed dye solution of 0.8% Lucifer yellow and 0.02% propidium iodide in CMF-PBS, and then monitored for evidence of Lucifer yellow dye transfer to adjoining cells using procedures previously described (Criswell et al., 1995). Because of its low molecular weight and hydrophilicity, Lucifer yellow readily diffuses between cells through connexin43 gap junctions but does not cross the non-gap junction plasma membrane of healthy cells. In contrast, propidium iodide rapidly binds to nucleic acids and serves as a marker to label injected cells. An injection pressure of 6.5 psi for 200 msec was used for dye injection. Gap junction communication was determined by visual examination 510 min after injection with an epifluorescence microscope (Nikon Diaphot) for Lucifer yellow dye fluorescence in cells adjacent to and in direct contact with the injected cell. Dye transfer was quantified as follows:
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Culture dishes were randomly assigned to treatment groups and utilized for one time-point only.
Measurement of cellular thiols.
High performance liquid chromatography (HPLC) with electrochemical detection was used to assay cellular GSH and GSSG in myometrial cells exposed to lindane. To prepare samples for HPLC analysis, the incubation medium was decanted from myometrial cell cultures, and the attached cells were quickly rinsed three times with pre-warmed CMF-PBS before cell lysis in 0.05 N perchloric acid. After collecting the lysate using a cell scraper, a small aliquot was set aside for protein analysis and the remainder was filtered through a 0.22-µm Acrodisc. The lysate and filtrate samples were flash-frozen in liquid nitrogen and stored at 70°C until HPLC and protein analysis. After thawing, the filtrate samples were separated with a C18 5 µ MF-Plus HPLC column (Alltech Assoc., Deerfield, IL) using a mobile phase consisting of 50 mM sodium dihydrogen phosphate (monohydrate), 0.05 mM 1-octanesulfonic acid (sodium salt), and 2% acetonitrile, adjusted to pH 2.70 with phosphoric acid. A Coulochem II electrochemical detector (ESA, Inc., Chelmsford, MA) monitored GSH and GSSG simultaneously in individual samples. Some samples were below the HPLC detection limit of GSSG (3 ng), and these samples were assigned the mid-value between zero and the detection limit value, i.e., 1.5 ng. The protein content of each HPLC sample was measured using the Bradford method (Bradford, 1976) as modified for use with a microtiter plate spectrophotometer, and cellular concentrations of GSH and GSSG were expressed as µg/mg protein. For those samples with GSSG concentrations below the limit of detection, 1.5 ng (the assigned GSSG value) was divided by the HPLC sample protein (expressed in mg).
Quantification of S-glutathionylation.
Evaluation of S-glutathionylation was based upon the method of Lou et al. (1986) as modified by Hiranruengchok and Harris (1995)
. Myometrial cell cultures were exposed to 50 or 100 µM lindane or to 0.1% DMSO (solvent control) in RPMI medium containing 10% BCS for 1 h at 37°C in a 5% CO2 atmosphere. The cells were then rinsed with prewarmed CMF-PBS, drained, and quickly scraped in 200 mM methanesulfonic acid. The cell suspensions were flash frozen using liquid nitrogen and stored at 70°C. Thawed cell and tissue samples underwent ultrasonic cell disruption while on ice, and protein was precipitated by addition of 4 M sodium methanesulfonic acid. Samples were centrifuged for 5 min at 150 x g at 4 °C. Protein pellets were washed with ice-cold 80% ethanol and were suspended in sodium pyrophosphate (pH 8.4). An enzymatic reduction system (5 mM EDTA, 1 mM dithiothreitol, 0.2 mM NADP+, 2.5 mM glucose-6-phosphate, 2 µg/ml glucose-6-phosphate dehydrogenase [Leuconostoc mesenteroides] and 4 µg/ml GSSG reductase [from Baker yeast]) was added to the protein suspension, and samples were incubated for 30 min at 37°C to reduce disulfide bonds and release free GSH. Upon cooling to room temperature, methanesulfonic acid was added at a final concentration of 200 mM to stop the reaction. Next, protein was precipitated by adding an equal volume of 4 M sodium methanesulfonic acid. Samples were centrifuged and supernatants were transferred to tubes containing HEPPS buffer (1 M HEPPS and 5 mM diethylene triamine, pH 8.5). S-Glutathionylation was quantified as the amount of GSH released in the supernatant. The GSH amounts in each sample were evaluated using HPLC with fluorometric detection as described by Fahey and Newton (1987)
and modified by Harris (1993)
. Samples were derivitized with monobromobimane solution at a final concentration of 0.2 mM and held in a dark environment at room temperature for 20 min. Methanesulfonic acid (400 mM) was then added to stop the reaction, and derivitized samples were stored at 70°C away from light until assayed by HPLC. Thiol analysis was conducted as described by Harris (1993)
using a scanning fluorescence detector. Following solubilization of the protein pellets set aside from each sample, protein values were determined using the Bradford assay (Bradford, 1976
) modified for use with a microtiter plate spectrophotometer. The amount of S-glutathionylation was expressed as nmoles of resolved GSH per mg protein.
Statistical analysis.
Data are reported as the mean ± standard error of the mean (SEM). Data analysis was conducted using SigmaStat (Jandel Scientific Software, San Rafael, CA) or Prism (GraphPad Software, Inc., San Diego, CA). Lindane-induced time-dependent changes in dye transfer were analyzed by two-way analysis of variance (ANOVA) with and without arcsine transformation of the data (to correct for non-normal distribution), and the results of the analyses were unaffected by the transformation. The HPLC measurements of GSH were analyzed by two-way ANOVA followed by post-hoc comparisons of means using the Student-Newman-Keuls test. The GSSG data set was not normally distributed because samples below the limit of GSSG detection were assigned the mid-value between zero and the detection limit value. Consequently, the GSSG and GSH/GSSG ratio data were analyzed using the distribution-free Mann-Whitney Rank Sum Test to compare control and lindane-treated cells at each time-point. The S-glutathionylation data were analyzed by one-way ANOVA followed by post-hoc comparisons of means using Student-Newman-Keuls pairwise multiple comparison tests. The diamide and BCNU data were analyzed by the Mann-Whitney Rank Sum Test. A p-value less than or equal to 0.05 was considered statistically significant.
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RESULTS |
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To more completely ascertain lindane modulation of cellular redox status, ratios of GSH/GSSG were determined by calculating the mean of individual sample GSH/GSSG ratios at each time-point from the data shown in Figures 3A and 3B. Immediately after a 1-h exposure to 100 µM lindane, the GSH/GSSG ratios decreased to an average of 0.98 compared with an average ratio of 17.5 in control cells (Fig. 3C, 0-h time-point; p 0.03). By 0.5 h after termination of lindane exposure, GSH/GSSG ratios partially recovered to 10.3 in lindane-exposed cells but still remained significantly depressed compared with 18.4 in control cells (Fig. 3C; p
0.03). Complete recovery of GSH/GSSG ratios to control levels was observed 1 h after removal of the lindane exposure medium and rinsing. However, 24 h after removal of lindane, GSH/GSSG ratios decreased again to 1.88 in lindane-exposed cells compared with a ratio of 18.3 in control cells (Fig. 3C; p
0.03). The GSH/GSSG ratios changed a biphasic manner that paralleled the patterns of lindane-induced inhibition of Lucifer yellow dye transfer and depression of cellular GSH.
Lindane-Induced Formation of S-Glutathionylation
Because lindane promoted oxidative cellular conditions immediately after a 1-h exposure, as indicated by the markedly reduced GSH/GSSG ratios at 0 h of recovery, the ability of lindane to promote S-glutathionylation under similar acute exposure conditions was determined. A 1-h exposure to 50 or 100 µM lindane stimulated S-glutathionylation in a concentration-dependent manner (Fig. 4; ANOVA treatment effect, p < 0.0001). S-Glutathionylation levels were low in control cells, as expected (averaging 0.20 nmoles released GSH/mg protein). However, lindane increased S-glutathionylation after a 1-h exposure to 50 or 100 µM lindane (1.6 and 3.4 nmoles released GSH/mg protein, respectively; significantly increased compared with controls, p 0.05). Consequently, S-glutathionylation was induced immediately after an acute (1-h) exposure to lindane under experimental conditions in which the GSH/GSSG ratios were markedly depressed.
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DISCUSSION |
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Exposure to the insecticide lindane (-hexachlorocyclohexane) inhibits gap junction intercellular communication between myometrial cells as assessed by Lucifer yellow dye transfer, consistent with previous reports in various cell types (Criswell et al., 1995
; Ruch and Klaunig, 1986
; Tsushimoto et al., 1983
). Confirming our previous observations (Krieger and Loch-Caruso, 2001
; Loch-Caruso et al., 2003
), an initial rapid recovery followed termination of a brief exposure to lindane, with the subsequent development of a secondary, delayed-onset inhibition of gap junction communication. The present study extended previous reports by showing continued inhibition of myometrial gap junctions for 96 h after termination of lindane exposure. In contrast to myometrial cells, rat liver WB-F344 cells completely recover from inhibition of gap junction communication 4 h after discontinuation of a 4-h exposure to lindane (Guan et al., 1995
). Differences between myometrial cells and WB-F344 cells in recovery from lindane-induced inhibition of gap junctions may be related to differences in phosphorylation of connexin43 at the protein kinase C phosphorylation site of serine 368 (Loch-Caruso et al., 2004
).
Cellular concentrations of GSH and GSSG in control myometrial cells were similar to uterine GSH and GSSG levels reported in literature (Suojanen et al., 1980), suggesting that the myometrial cell cultures maintained GHS/GSSG homeostasis in vitro similar to that observed in vivo. A brief (1-h) exposure to lindane acutely depleted GSH of cultured myometrial cells, consistent with reports that lindane reduces GSH in rat liver (Barros et al., 1988
; Videla et al., 1990
) and in rat embryos and visceral yolk sac (McNutt and Harris, 1994
), and providing the first report of GSH depletion in myometrium in response to lindane. Furthermore, the present report provides the first demonstration of a lindane-induced biphasic effect on cellular GSH, characterized by recovery of cellular GSH to control levels within 1 h after termination of lindane exposure, and then the redevelopment of a secondary, delayed-onset decline of GSH observed 24 h after discontinuation of exposure to lindane. The lindane-induced changes in myometrial GSH followed a similar temporal pattern as inhibition of myometrial gap junction communication, suggesting that depletion of cellular GSH may be involved in lindane's acute and delayed-onset inhibition of myometrial gap junctions. Decreased cellular GSH was correlated with diminished gap junction intercellular communication in rat-1 fibroblast variants (Masta et al., 1991
) and in liver cell lines (Barhoumi et al., 1993
), also.
After a brief (1-h) exposure to lindane, cellular GSSG varied in a biphasic manner that was inversely related to GSH, suggesting that GSH depletion was linked to oxidation of GSH to GSSG. Moreover, lindane depressed GSH/GSSG ratios in a manner that paralleled changes of cellular GSH, providing additional support that lindane promoted GSH oxidation to GSSG. Because the GSH/GSSG pattern varied in a similar manner as inhibition of gap junctions, oxidation of GSH to GSSG may be related to lindane-induced inhibition of myometrial gap junctions.
The GSH/GSSG ratio is an excellent indicator of cell redox status (Schafer and Buettner, 2001). As such, the markedly depressed GSH/GSSG ratios observed immediately after a 1-h exposure to lindane is consistent with increased generation of superoxide and induction of oxidative stress previously observed in myometrial cells exposed to lindane under identical conditions (Caruso et al., 2005
; Krieger and Loch-Caruso, 2001
). Moreover, oxidative stress has been reported in liver cells exposed to lindane (Videla et al., 1990
). Increased generation of superoxide, as was observed in myometrial cells under identical lindane exposure conditions (Caruso et al., 2005
), would be expected to promote oxidation of cysteines of cellular proteins and subsequent S-glutathionylation. The present study provides the first report that lindane stimulates S-glutathionylation and is the first to associate S-glutathionylation with inhibition of gap junctions.
Because S-glutathionylation most likely occurs by direct reaction of GSH with an oxidized protein cysteine, the finding that lindane increased S-glutathionylation is consistent with cellular oxidative stress (Mannervik et al., 1989; Poole et al., 2004
) and suggests a potential mechanism whereby lindane may acutely deplete cellular GSH. Moreover, S-glutathionylation may occur by direct reaction of GSSG with a protein thiol(ate) (see also Poole et al., 2004
). Consequently, the elevated GSSG and reduced GSH/GSSG ratios observed immediately after a brief (1-h) exposure to lindane could also contribute to the increased S-glutathionylation observed in myometrial cells under identical lindane exposure conditions.
Consistent with the reversibility of S-glutathionylation by thioredoxin, glutaredoxin, or protein disulfide isomerase systems (Poole et al., 2004), GSH concentrations were restored to control levels 1 h after termination of lindane exposure in myometrial cells. Although initial recovery of GSH after discontinuation of lindane treatment theoretically could be the result of de novo synthesis of GSH, the rapid rate of recovery of GSH pools makes de novo synthesis unlikely. Moreover, lack of stoichiometry between GSSG and GSH levels suggests that regeneration of GSH from reduction of GSSG by NADPH-dependent GSSG reductase is an unlikely explanation for the initial recovery of GSH. Consequently, S-glutathionylation provides a plausible explanation for cellular GSH depletion during lindane exposure and, through its rapid reversal by thioredoxin, glutaredoxin, or protein disulfide isomerase, S-glutathionylation may also explain the initial recovery of GSH observed 1 h after termination of lindane exposure.
Because the antioxidant and GSH modulation treatments that prevented the delayed-onset inhibition of gap junctions in previous studies were pre-/cotreatments with a 1-h lindane exposure, the lindane-induced delayed-onset inhibition of myometrial gap junctions likely is dependent on acute oxidative stress during the 1-h lindane exposure (Caruso et al., 2005; Krieger and Loch-Caruso, 1997
). S-Glutathionylation was assessed in the present study and indices of oxidative stress were measured in previous studies (Caruso et al., 2005
; Krieger and Loch-Caruso, 1997
) immediately after lindane exposure because the available evidence suggested that the critical events were initiated during the 1-h lindane exposure. Nonetheless, it may be interesting to measure oxidative stress by means other than GSH and GSSG at various times after termination of lindane exposure, in order to better interpret the delayed-onset reductions of GSH and GSH/GSSG ratios. These studies are beyond the scope of the present investigation, however.
The development of secondary, delayed-onset decreases of GSH and GSH/GSSG ratios observed 24 h after cessation of a brief (1-h) lindane exposure suggest that a GSH-related mechanism is initiated during exposure to lindane that requires time to develop. A change of cellular redox status, as evidenced by depressed GSH/GSSG ratios immediately after a 1-h exposure to lindane, may modify protein expression of redox regulated genes (Allen and Tresini, 2000; Rahman et al., 2005
) that, in turn, leads to the development of a secondary depletion of GSH and inhibition of gap junctions. A gene transcription-dependent process would be expected to require more than 1 h to develop, consistent with the delayed onset of the secondary inhibition of myometrial gap junctions. However, investigation of this mechanism requires further experimentation beyond the present study.
Alternatively, both the initial and delayed-onset inhibition of myometrial gap junctions by lindane may involve S-glutathionylation of connexin43, the gap junction protein abundantly expressed in the myometrium during parturition (Risek et al., 1990) and in myometrial cells in culture (Caruso et al., 1990
). Because connexin43 has six extracellular cysteines that are critical for channel function (John and Revel, 1991
) and three cysteines located on the cytoplasmic carboxy terminus, the connexin43 cysteines may become oxidized and glutathionylated under conditions of oxidative stress with consequential alteration of protein function, as observed with other proteins (Poole et al., 2004
). The inhibition of myometrial gap junctions observed immediately after a 1-h exposure to lindane was shown to be dependent on cellular GSH (Caruso et al., in press), consistent with a role for S-glutathionylation in development of acute inhibition of myometrial gap junctions. Although S-glutathionylation is readily reversible, the more oxidized forms of protein cysteines (e.g., sulfenate, sulfinate, and sulfonate) are less so and may be irreversible (Poole et al., 2004
). It is suggested that S-glutathionylation, which occurs under acute lindane exposure conditions as shown by the present study, is mechanistically related to the acute inhibition of myometrial gap junctions, and that further, less readily reversible, oxidation of cell protein cysteines may develop over a longer period and possibly underlie the development of the secondary, delayed-onset inhibition of gap junctions. Although our data are consistent with this explanation, further study is required to examine long-term oxidative effects of lindane on cell proteins critical for gap junction regulation.
Treatment with diamide depressed myometrial gap junction intercellular communication, consistent with previous reports that diamide decreases gap junctional electrical coupling in crayfish giant axons (Campos de Carvalho et al., 1986) and augments phorbol ester-induced inhibition of gap junctions in WB-F344 rat liver cells (Hu and Cotgreave, 1995
). Because diamide directly and reversibly oxidizes GSH to GSSG without formation of radicals (Kosower and Kosower, 1976
), the rapid inhibition of myometrial gap junction communication by diamide implicates a role for GSH oxidation to GSSG in myometrial gap junction inhibition. Similar to diamide, the GSSG reductase inhibitor 1,3-bis(2-chloroethyl)-1-nitrosourea (BCNU) inhibited myometrial gap junction communication. Because BCNU promotes cellular increases of GSSG by preventing reduction of GSSG to GSH, the ability of BCNU to inhibit myometrial gap junctions further suggests a role for GSSG in the regulation of myometrial gap junctions. To our knowledge, this is the first report that BCNU inhibits gap junctions and the first evidence supporting GSH oxidation as a more general regulatory mechanism of myometrial gap junctions.
A previous study in our laboratory suggested that lindane inhibits myometrial gap junctions and spontaneous oscillatory contractions by a phospholipase C-mediated mechanism (Wang and Loch-Caruso, 2002). Additional preliminary experiments further suggest that lindane's mechanism of inhibition of myometrial gap junctions is mediated by PKC
-dependent activation of NADPH oxidase (Wang and Loch-Caruso, 1999
). NADPH oxidase activation could be a mechanism by which lindane exposure leads to GSH oxidation in myometrial cells because lindane increases generation of superoxide (Caruso et al., 2005
), NADPH oxidase activation increases superoxide production, and superoxide promotes GSH oxidation to GSSG.
Lindane greatly increases release of arachidonic acid from myometrial cells. Because arachidonic acid metabolism stimulates conversion of GSH to GSSG (Burch and Burch, 1990), release of arachidonic acid could initiate the lindane-induced GSH oxidation observed in the present study. However, an arachidonic acid metabolism-mediated mechanism does not appear to link lindane-induced oxidation of GSH to inhibition of gap junctions because the cyclooxygenase inhibitor indomethacin has only a marginal impact on lindane-induced inhibition of myometrial gap junctions (Criswell and Loch-Caruso, 1995
). Lindane activates cAMP and calcium cell signaling pathways in myometrial cells, also, but a role for these signaling molecules in lindane-induced inhibition of myometrial gap junctions was not supported by experimental results (Criswell et al., 1994
, 1995
; Criswell and Loch-Caruso, 1995
, 1999
).
Inhibition of gap junction intercellular communication has been linked to tumorigenesis, impaired uterine contraction, and other pathophysiologic phenomena (Loch-Caruso, 1999; Trosko and Chang, 2000
). Furthermore, lindane-induced inhibition of myometrial gap junctions and spontaneous uterine contractions is prevented by antioxidant treatments (Krieger and Loch-Caruso, 2001
), consistent with a critical role for oxidative stress-mediated inhibition of myometrial gap junctions in the dysregulation of uterine contractions. Although gap junctions serve to improve uterine muscle coordination and force generation at parturition (Garfield et al., 1978
; Garfield and Hayashi, 1981
), it is not known whether lindane presents reproductive risks to women by inhibiting myometrial gap junctions and uterine contractions during pregnancy. The concentration of lindane used in the present study is about 100-fold higher than serum concentrations reported in humans after occupational exposure (Baumann et al., 1980
) or pharmaceutical use of lotion containing 1% lindane (Rauch et al., 1990
). However, because lindane induces an inhibition of myometrial gap junctions that is sustained for at least four days after discontinuation of exposure (Loch-Caruso et al., 2003
), further research on possible health impacts in pregnant women may be warranted. However, it is beyond the scope of the present investigation to resolve whether lindane poses a reproductive risk to pregnant women by interfering with myometrial gap junctions.
The parallel nature of lindane-induced inhibition of gap junction communication, GSH depletion and GSH/GSSG ratio decrease suggest that GSH oxidation to GSSG may be part of the mechanism by which lindane inhibits myometrial gap junction communication. Moreover, the data suggest a role for S-glutathionylation in lindane's biphasic effects on myometrial GSH/GSSG and gap junction communication. Finally, inhibition of myometrial gap junctions by pharmacological treatments that elevate the ratio of GSH/GSSG suggest that the GSH/GSSG redox couple may serve as a more general regulatory mechanism of myometrial gap junctions. A mechanism by which S-glutathionylation could regulate gap junctions under conditions of GSH oxidation to GSSG is proposed, but elucidation of the exact mechanism remains beyond the scope of the present investigation.
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ACKNOWLEDGMENTS |
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