Calcium/calmodulin-dependent protein kinase II links ER stress with Fas and mitochondrial apoptosis pathways (original) (raw)
Fas, an important protein in macrophage apoptosis during cholesterol loading, is induced by ER stress in a calcium-dependent manner. Our initial goal was to determine whether there is a mechanistic link between 2 processes previously shown to be involved in ER stress–induced macrophage apoptosis, namely, calcium-CaMKII signaling and activation of the Fas pathway (10, 23, 25). As a model of ER stress–induced apoptosis, macrophages were incubated under conditions promoting the accumulation of lipoprotein-derived cholesterol (3, 10, 11). In our original Fas study (10), a serum-deprivation component was included in the model, but we have since cultured the macrophages in full serum in order to simplify the conditions. In the current model, we first determined the role of Fas in apoptosis. Macrophages from Lpr mice, which lack Fas receptors, showed a 60% reduction in cholesterol-induced apoptosis compared with macrophages from WT mice (P = 0.01; Figure 1A). Inhibition of caspase-8, the downstream caspase of Fas, with Z-Ile-Glu(OMe)-Thr-Asp-fluoromethylketone inhibited cholesterol-induced apoptosis from 17.9% ± 1.5% to 8.5% ± 0.9% (P < 0.001). We then tested whether cholesterol loading affected expression of Fas itself, and found that cholesterol loading led to a marked induction of Fas mRNA (Figure 1B) and total and cell surface Fas protein (Figure 1C). The latter finding, which was obtained using a cell surface biotinylation protocol, is important because Fas is active in apoptotic signaling as a cell-surface receptor (27). Thus, cholesterol loading of macrophages induces Fas expression, which plays a proapoptotic role in these cells.
Proapoptotic Fas is induced by ER stress in a calcium-dependent manner. (A) Peritoneal macrophages from WT or Lpr mice were incubated for 14 hours under control (Con) or cholesterol-loading (Chol) conditions. Mid- and late-stage apoptosis were assayed using Alexa Fluor 488–conjugated annexin V (green) and PI (orange-red), respectively. Scale bar: 20 μm. For each group, 3 fields were quantified and expressed as a percentage of annexin/PI-positive cells. Mϕ, macrophage. (B) Macrophages from WT mice were incubated under cholesterol-loading conditions for the indicated times. Fas mRNA, measured using quantitative PCR, is expressed relative to internal control mRNA. (C) Macrophages were incubated for 8 hours under control, cholesterol-loading, or cholesteryl ester–loading (CE) conditions and then assayed for total and cell surface Fas protein by immunoblot following biotinylation of cell surface proteins. Hsp90 was used as a cytosolic marker, and β1 integrin as a cell surface marker and loading control. (D and E) Macrophages were incubated under control or cholesterol-loading conditions or with 0.25 μM thapsigargin (Thaps) and then assayed for Fas mRNA and protein. (F and G) Macrophages were incubated under control or cholesterol-loading conditions in the absence or presence of the cholesterol trafficking inhibitor U18666A (U18) after 1 hour pretreatment with the compound, and then assayed for Fas mRNA and protein. (H and I) Macrophages were incubated under control or cholesterol-loading conditions with BAPTA-AM or equivalent volumes of vehicle (Veh) control after 1 hour pretreatment, and then assayed for Fas mRNA and protein. Differing symbols indicate P < 0.01; identical symbols indicate differences that are not significant.
Lipoprotein-mediated cholesterol loading induces apoptosis through 2 proapoptotic hits: ER stress induced by lipoprotein-derived cholesterol and additional death signaling through engagement of PRRs by the lipoproteins themselves (12, 15, 23). The first evidence that the ER stress hit was important in Fas induction was our finding in Figure 1C that induction of Fas protein was not observed in macrophages incubated under conditions in which lipoprotein cholesterol is efficiently esterified to fatty acids, which do not perturb the ER membrane and thus do not cause ER stress (3). Second, we found that the sarcoplasmic/endoplasmic reticulum calcium-dependent ATPase (SERCA) inhibitor thapsigargin, a UPR activator, induced Fas mRNA and protein (Figure 1, D and E). Third, we took advantage of the fact that the steroid 3β-[2-(diethylamino)ethoxy]-androst-5-en-17-one hydrochloride (U18666A) blocks the trafficking of lipoprotein-derived cholesterol from late endosomes to the ER and thus prevents cholesterol-induced ER stress and apoptosis (3). Loading macrophages with cholesterol in the presence of U18666A suppressed Fas mRNA and protein to basal levels (Figure 1, F and G). As a control, we showed that Fas induction by LPS, a non-ER stress inducer of Fas (28), was not blocked by U18666A (data not shown). Thus, ER stress is essential for Fas induction during enrichment of macrophages with lipoprotein-cholesterol.
A critical mechanism by which ER stress enables apoptosis in macrophages is through release of ER calcium stores into the cytosol (23, 25). To determine the role of cytosolic calcium in cholesterol-mediated Fas induction, macrophages were loaded with cholesterol in the absence or presence of a cytosolic calcium chelator, 1,2-bis(2-aminophenoxy)ethane-N,N,_N_′,_N_′-tetraacetate–AM (BAPTA-AM). Our previous work showed that BAPTA-AM blocks cholesterol-induced apoptosis (23). BAPTA-AM almost completely prevented Fas mRNA and protein induction (Figure 1, H and I), suggesting a critical role for cytosolic calcium in this process. In summary, ER stress, including that induced by cholesterol loading, induces Fas, which is an important protein in ER stress–induced macrophage apoptosis. Cytosolic calcium, a key agent in ER stress–induced apoptosis (23, 25), is required for this process.
Cholesterol loading leads to sustained activation of CaMKII. CaMKII is a critical signal transducer in ER stress–induced macrophage apoptosis (25) and thus was a candidate for mediating calcium-dependent induction of Fas. We first sought to firmly establish that CaMKII was activated in this model. Macrophages were incubated under cholesterol-loading conditions for various times, and then cell extracts were assayed for their ability to transfer 32P from [γ–32P]ATP to the CaMKII-specific substrate, KKALRRQETVDAL (29). CaMKII activity increased steadily as a function of time of cholesterol loading up to 7 hours (Figure 2A). As a negative control, 4-hour cells were incubated with the specific CaMKII peptide inhibitor autocamtide-2–related inhibitory peptide II (AIP-II), which contains the sequence of the Thr287-containing autophosphorylation domain and thus acts as a competitive inhibitor of autophosphorylation (30); and the calcium chelator EGTA was added in vitro to the enzyme reaction mix. CaMKII activity was very low under these conditions (Figure 2A, asterisk). A repeat experiment at the 6-hour time point again showed activation of the enzyme (Figure 2B).
Cholesterol loading leads to sustained activation of CaMKII. (A) CaMKII activity was assayed in individual wells of macrophages incubated under cholesterol-loading conditions for the indicated times. The asterisk indicates CaMKII activity from cells loaded with cholesterol for 4 hours in the presence of 10 μM AIP-II (EGTA was included during the assay). (B) CaMKII activity was assayed in triplicate wells of macrophages incubated under control or cholesterol-loading conditions for 6 hours. Differing symbols indicate P = 0.001. (C) Top: Macrophages were incubated under control or cholesterol-loading conditions with BAPTA-AM or vehicle after 1 hour pretreatment, and lysates were then immunoblotted for phospho-CaMKII, total CaMKII, and β-actin. Bottom: As above, except ER stress was induced with 3 μg/ml tunicamycin (Tun). (D) Macrophages were incubated under control or cholesterol-loading conditions with or without 10 μM AIP-II after 1 hour pretreatment, and lysates were then immunoblotted for phospho-CaMKII, total CaMKII, and β-actin. (E and F) As in D, except that (E) ER stress was induced with 0.25 μM thapsigargin, or (F) 10 μM KN93 was used as the CaMKII inhibitor, with 10 μM KN92 as the inactive analog. (G) In 2 independent experiments, macrophages were incubated under control or cholesterol-loading conditions. CaMKII was then immunoprecipitated from cell lysates using anti-CaMKII or control IgG (bottom). The immunoprecipitates were then blotted for oxidized CaMKII using anti–Ox-CaMKII antiserum and total CaMKII.
CaMKII is initially activated by calcium/calmodulin through transient increases in cytosolic calcium, leading to sustained, calcium-independent activity due to inactivation of the autoinhibitory domain of the enzyme through autophosphorylation at Thr287 (31). Thus, another measure of CaMKII activation is the appearance of phospho–Thr287 CaMKII. There was an increase in phospho-Thr287 CaMKII at relatively early time points of cholesterol loading (Figure 2C), consistent with this process leading to sustained enzyme activation at later time points (see above and ref. 25). Although there was some variability among experiments as to the exact timing of onset and duration of phospho-CaMKII after cholesterol loading, we consistently observed its appearance within 30–60 minutes of cholesterol loading, with a duration of 2–6 hours. Another inducer of ER stress is the glycosylation inhibitor tunicamycin, and treatment of macrophages with this reagent also caused a marked increased in CaMKII phosphorylation. To validate phospho-CaMKII as a marker of CaMKII activation in our models, we tested the effect of BAPTA-AM, which should block the interaction of calcium with calmodulin and thus prevent phosphorylation of the enzyme. Consistent with this point, we found that BAPTA-AM markedly decreased both cholesterol- and tunicamycin-induced CaMKII phosphorylation (Figure 2C).
We next used phospho-CaMKII to further validate the use of AIP-II as a CaMKII inhibitor (above) as well as another, structurally unrelated CaMKII inhibitor, 2-[N-(2-hydroxyethyl)]-N-(4-methoxybenzenesulfonyl)]amino-N-(4-chlorocinnamyl)-N-methylbenzylamine (KN93), that we used in the following experiments. As expected from the data in Figure 2A, AIP-II blocked both cholesterol- and thapsigargin-induced CaMKII phosphorylation (Figure 2, D and E). Note that CaMKII phosphorylation occurred at a much earlier time point with thapsigargin than with lipoprotein-cholesterol loading, as expected of a direct SERCA inhibitor. Cholesterol-induced CaMKII phosphorylation was also blocked by KN93, but not by its inactive homolog, [N-(4-methoxybenzenesulfonyl)]amino-N-(4-chlorocinnamyl)-N-methylbenzylamine phosphate (KN92; Figure 2F). These combined data show that a variety of ER stressors activate CaMKII in macrophages and validate the use of AIP-II and KN93 as CaMKII inhibitors in these models (see below).
Prolonged ER stress can generate intracellular ROS (4), and recent work in our laboratory has shown that cholesterol loading is a potent inducer of ROS in macrophages (G. Li, unpublished observations; T.A. Seimon, unpublished observations). Erickson et al. (32) recently showed that ROS-mediated oxidation of Met281/282 in the autoinhibitory domain of CaMKII further prolongs CaMKII activity after an initial calcium transient by a mechanism analogous to autophosphorylation. We therefore probed immunoprecipitated CaMKII in cholesterol-loaded macrophages with an antibody specific for the oxidized CaMKII regulatory domain peptide M281/282 (Ox-CaMKII). In 3 independent experiments, we found a positive Ox-CaMKII signal after 2 hours of cholesterol loading (Figure 2G). Thus, cholesterol loading leads to sustained activation of CaMKII, which likely involves initial activation by cytosolic calcium followed by prolonged activation through autophosphorylation- and oxidation-mediated modification of the autoinhibitory domain.
Induction of Fas and apoptosis by ER stress involves CaMKII. Given the role of cytosolic calcium in cholesterol-induced Fas induction and the ability of cholesterol loading to activate CaMKII, we addressed the causative role of CaMKII in this process. Inclusion of the CaMKII inhibitor KN93 during cholesterol loading prevented Fas induction, whereas KN92 had no inhibitory effect (Figure 3A). To further substantiate this important point, we used a CaMKII siRNA knockdown approach. We first showed by RT-PCR that mouse peritoneal macrophages express only the γ isoform of CaMKII (Figure 3B) and then found 3 CaMKIIγ siRNA species that decreased CaMKII expression by 55%–75% (Figure 3C). Consistent with the KN93 data, cholesterol-induced Fas protein was suppressed by these siRNA species, whereas a scrambled siRNA had no effect (Figure 3C). Thus, CaMKII activity and expression are necessary for ER stress–mediated Fas induction
Induction of Fas and apoptosis by ER stress involves CaMKII. (A) Macrophages were incubated for 8 hours under cholesterol-loading conditions with or without KN93 or KN92 after 1 hour pretreatment, and then assayed for Fas mRNA. (B) RNA from peritoneal macrophages from 4 separate mice and from mouse brain, along with water control, were probed for the indicated CaMKII isoform mRNAs by RT-PCR. (C) Macrophages were transfected with 3 different CaMKIIγ siRNA constructs. After 72 hours, the cells were incubated for 8 hours under cholesterol-loading conditions and then assayed for CaMKIIγ mRNA and total Fas protein. (D) Macrophages were transfected with the 3 siRNA constructs in C, incubated for 30 hours with 0.25 μM thapsigargin and 25 μg/ml of the SRA ligand fucoidan, and then assayed for apoptosis. (E) Macrophages from WT or Camk2g–/– mice were incubated under control or cholesterol-loading conditions for 12 hours and then assayed for apoptosis. Scale bar: 20 μm. (F) Human aortic endothelial cells were incubated for 24 hours with thapsigargin (1 μM) with or without KN93 or KN92 after 1 hour pretreatment, and then assayed for apoptosis. (G) PC12 cells were incubated for 24 hours with 100 μM 6-OHDA with or without 10 μM AIP-II after 1 hour pretreatment, and then assayed for cell viability (percentage of viable cells compared with those in cultures not treated with 6-OHDA). Differing symbols indicate P < 0.01; identical symbols indicate differences that are not significant.
The role of CaMKII in ER stress–induced Fas induction would predict that the kinase plays a critical role in ER stress–induced apoptosis. In a previous study, we showed that KN93 blocked cholesterol-induced macrophage apoptosis (25). Our goal here was to substantiate this important finding through genetic targeting of CaMKIIγ. First, we used the active siRNA species described above and found that knockdown of CaMKIIγ suppressed cholesterol-induced apoptosis (Figure 3D). Second, cultured peritoneal macrophages derived from Camk2g–/– mice showed no detectable CaMKIIγ protein by immunoblot (below). We found that cholesterol-induced apoptosis was suppressed in CaMKIIγ-deficient macrophages to a degree similar to that found using the siRNA approach (Figure 3E).
To broaden the implications of our findings, we tested the role of CaMKII in ER stress–induced apoptosis using 2 additional models. The endothelium of advanced atheromata displays markers of UPR activation (17). Using thapsigargin-treated human aortic endothelial cells as a model, we showed that apoptosis under these conditions was markedly suppressed by KN93, but not by KN92 (Figure 3F). In a completely different model, we examined apoptosis of the neuronal cell line PC12 by 6-hydroxydopamine (6-OHDA), a model of Parkinson disease that has previously been shown to be mediated through activation of the UPR (33). We found that 6-OHDA decreased the survival of PC12 cells, and this effect was prevented by about 50% by pretreatment with AIP-II (P < 0.01; Figure 3G). KN93 also suppressed 6-OHDA–induced apoptosis in PC12 cells (data not shown). These data show that CaMKII is involved in ER stress–induced apoptosis in a number of different scenarios.
JNK mediates the proapoptotic role of CaMKII in ER-stressed macrophages. Reports in the literature have suggested links between CaMKII and JNK (34, 35), and between JNK and Fas induction (36, 37). Moreover, we reported that JNK is activated by and necessary for apoptosis in ER stress–induced macrophages (15). We therefore hypothesized the presence of a CaMKII-JNK-Fas pathway. To determine a possible role for JNK in cholesterol-mediated Fas induction, macrophages were loaded with cholesterol in the absence or presence of the JNK inhibitor SP600125. The JNK inhibitor prevented the induction of Fas mRNA and protein in the cholesterol-loaded cells (Figure 4, A and B). To confirm these results, macrophages from WT mice and from mice lacking JNK2, the predominant form expressed in macrophages (15), were loaded with cholesterol and assayed for Fas mRNA and protein. Fas induction was markedly suppressed in Jnk2–/– macrophages (Figure 4, C and D). Next, we determined whether CaMKII was upstream of JNK activation. Inhibition of CaMKII in cholesterol-loaded macrophages by AIP-II blocked JNK phosphorylation (Figure 4E). Similar results were found when CaMKII was inhibited by KN93 (data not shown). AIP-II did not inhibit LPS-induced JNK phosphorylation (Figure 4F), indicating that AIP-II is not simply a general inhibitor of JNK activation. In considering possible mechanisms through which CaMKII might activate JNK, we probed the upstream JNK kinase mitogen-activated protein kinase kinase–4 (MKK4) for CaMKII-dependent phosphorylation. Cholesterol loading was associated with an increase in the phosphorylation of MKK4, and phosphorylation was markedly suppressed by treatment of the cells with AIP-II (Figure 4E). The upstream kinase MKK7 was not phosphorylated by cholesterol loading of macrophages (data not shown). Cultured peritoneal macrophages derived from Camk2g–/– mice, which showed no detectable CaMKIIγ protein by immunoblot, also responded to cholesterol loading with substantially less induction of Fas, phospho-JNK, and phospho-MKK4 than macrophages from WT mice (Figure 4G). In summary, the combined data in Figures 1–4 support a model in which ER stress triggers a critical apoptosis pathway involving CaMKII activation, which, through activation of JNK, and perhaps via activation of MKK4, induces proapoptotic Fas.
JNK mediates the proapoptotic role of CaMKII in ER-stressed macrophages. (A and B) Macrophages were incubated under control or cholesterol-loading conditions with or without 10 μM of the JNK inhibitor SP600125 after 1 hour pretreatment, and then assayed for Fas mRNA (A) and protein (B). (C and D) Macrophages from WT or Jnk2–/– mice were incubated under control or cholesterol-loading conditions and then assayed for Fas mRNA (C) and protein (D). (E) Macrophages were incubated under control or cholesterol-loading conditions for 4 hours with or without 10 μM AIP-II after 1 hour pretreatment. One aliquot of the cell extracts was immunoblotted for phospho-JNK, total JNK, and β-actin, and another was immunoblotted for phospho-MKK4 and β-actin. (F) Macrophages were incubated with 100 ng/ml LPS for the indicated times with or without 10 μM AIP-II after 1 hour pretreatment. Phospho-JNK and total JNK were then assayed by immunoblot. (G) Macrophages from WT or Camk2g–/– mice were incubated under control or cholesterol-loading conditions and then immunoblotted for CaMKII, Fas, phospho-JNK, JNK, phospho-MKK4, MKK4, and β-actin. Differing symbols indicate P < 0.01; identical symbols indicate differences that are not significant.
Release of mitochondrial cytochrome c and loss of mitochondrial membrane potential in cholesterol-loaded macrophages is CaMKII dependent. We have previously shown that cholesterol loading leads to release of cytochrome c and induction of caspase 9–mediated apoptosis as well as loss of mitochondrial membrane potential (Δψm) (11). While the exact relationship between cytochrome c release, which is caused by outer mitochondrial membrane permeabilization, and Δψm is controversial and likely varies in different apoptotic scenarios, both events have been associated with apoptosis (38). In the context of the current study, we sought to determine whether there was a link between CaMKII signaling and these events in ER-stressed macrophages. We first verified that a key event in mitochondrial-mediated apoptosis, namely, Δψm, was present in the current serum-replete model of cholesterol-induced apoptosis. There was marked loss of MitoTracker Red staining, a marker of mitochondrial membrane potential, after 12 and 16 hours of cholesterol loading (Figure 5A). The loss of MitoTracker Red staining was prevented by treatment with KN93, but not by KN92 treatment (Figure 5A). Similar data were obtained when macrophages from Camg2g–/– mice were used instead of treating WT macrophages with KN93: the cholesterol-induced decrease in MitoTracker Red staining was much greater in WT than in CaMKIIγ-deficient macrophages (Figure 5B).
Release of mitochondrial cytochrome c and Δψm in cholesterol-loaded macrophages is dependent on CaMKII. (A) Macrophages were incubated under control or cholesterol-loading conditions for 12 or 16 hours in the absence or presence of 10 μM KN93 or KN92 after 1 hour pretreatment. Cells were then stained with MitoTracker Red and examined by confocal fluorescence microscopy. Mean fluorescence intensity per cell is also shown (n = 100 cells). (B) Macrophages from WT or Camk2g–/– mice were incubated under control or cholesterol-loading conditions for 12 hours and then assayed for MitoTracker Red staining. (C) Macrophages were treated for 8 hours as in A. Mitochondrial and cytosolic fractions were assayed for cytochrome c, tubulin (cytosolic marker), and prohibitin (mitochondrial marker). (D) Macrophages from WT or Stat1–/– mice were incubated under control or cholesterol-loading conditions for 12 or 16 hours and then stained with MitoTracker Red. (E) Macrophages were incubated under control or cholesterol-loading conditions for 16 hours in the absence or presence of 10 μM of the JNK inhibitor SP600125 after 1 hour pretreatment, and then stained with MitoTracker Red. Scale bars: 20 μm (A); 10 μm (D and E). Differing symbols indicate P < 0.01; identical symbols indicate differences that are not significant.
We next turned our attention to cytochrome c release. Cholesterol loading led to a loss of cytochrome c in the mitochondria and appearance in the cytosol (Figure 5C). This event was suppressed by KN93, but not by KN92 (Figure 5C). Note that the mitochondria were free of cytosolic contamination, as assessed by the absence of tubulin (Figure 5C) and of β-actin and GAPDH (data not shown). Thus, CaMKII signaling is necessary for Δψm and mitochondrial cytochrome c release during cholesterol-induced ER stress.
We recently showed that the proapoptotic signal transducer STAT1 was activated downstream of CaMKII in ER-stressed macrophages and was required for ER stress–induced macrophage apoptosis in vitro and for advanced lesional macrophage apoptosis and plaque necrosis in vivo (25). Moreover, in other systems, STAT1-induced apoptosis has been linked to the Δψm (39). To determine whether CaMKII-mediated Δψm was STAT1 dependent, we assayed MitoTracker Red staining in cholesterol-loaded macrophages from WT versus Stat1–/– mice. Cholesterol-induced loss of MitoTracker Red staining was completely unaffected by STAT1 deficiency (Figure 5D). We next considered the possibility that JNK might link CaMKII activation with Δψm, as it did in Fas induction (see above). However, inhibition of JNK did not block the decrease in MitoTracker Red staining in cholesterol-loaded macrophages (Figure 5E). Thus, CAMKII-mediated Δψm in ER-stressed macrophages involves a mechanism that is independent of both STAT1 and JNK signaling.
ER stress results in CaMKII-dependent accumulation of calcium in the mitochondria. A potential mechanism linking ER stress with proapoptotic mitochondrial dysfunction is excess transfer of calcium from ER stores into the mitochondria, leading to Δψm (40–42). To determine whether mitochondrial calcium uptake is increased in ER-stressed macrophages, macrophages were incubated under cholesterol-loading conditions for 1.5 hours, the last 30 minutes of which included loading the cells with the cytoplasmic fluorescent calcium sensor Fura-2. At the end of the incubation period, the cells were imaged for Fura-2 fluorescence and exposed to the uncoupling agent FCCP, which releases mitochondrial calcium into the cytoplasm. Thus, the post-FCCP increase in Fura-2 fluorescence is proportional to the content of mitochondrial calcium at the end of the cholesterol loading period (43). The fluorescence intensity of Fura-2 after FCCP treatment was substantially greater in cholesterol-loaded than in control macrophages (Figure 6A). As a control, we showed that cells under both conditions responded similarly to ionomycin-induced expansion of cytosolic calcium pools. This experiment was conducted on several fields of cells with similar results (data not shown). These data indicate that mitochondrial calcium content was increased by cholesterol loading.
ER stress in macrophages leads to the accumulation of calcium in the mitochondria. (A) Macrophages were plated on 25-mm coverslips and grown to confluency. The cells were incubated under control or cholesterol-loading conditions for 1 hour and stained with 5 μM Fura-2 for 30 minutes. The cells were then rinsed in medium and examined by fluorescence microscopy, where calcium fluorescence was measured every second. FCCP (1 μM), a mitochondrial uncoupler, and ionomycin (10 μM) were added at the indicated times to release mitochondrial and overall intracellular calcium stores, respectively. (B) Macrophages were treated with medium alone as control, with 0.25 μM thapsigargin for 1 hour, or under cholesterol-loading conditions for 2 or 4 hours. At the end of each incubation, 10 μM Rhod-2, a mitochondrial-specific fluorescent calcium dye, was added to the media, and the cells were incubated on ice for 1 hour at 4°C. The cells were then washed and incubated for an additional 5 hours with thapsigargin or under cholesterol-loading conditions, such that total incubation time for thapsigargin was 5 hours and for cholesterol 5 or 7 hours. At the end of the incubation period, the cells were visualized using confocal microscopy and imaged as described in Methods. Scale bar: 10 μm. Fluorescence intensity for approximately 100 cells was measured for each treatment group. Differing symbols indicate P < 0.01; identical symbols indicate differences that are not significant.
To corroborate our finding that mitochondrial calcium was increased by cholesterol, we assayed mitochondrial calcium by an alternative, direct method. We loaded cells with the calcium-sensitive fluorescent dye Rhod-2 under conditions in which the dye is sequestered in mitochondria (44). Rhod-2 has a net positive charge and therefore preferentially accumulates in the mitochondria. Moreover, the dye is loaded into the cells at 4°C to prevent cleavage of the ester as it traffics to the mitochondria, followed by incubation at 37°C to allow mitochondrial esterases to activate the dye (44). Both the ER stressor thapsigargin and cholesterol loading caused a marked increase in Rhod-2 fluorescence in macrophages (Figure 6B). Note that addition of type A scavenger receptor (SRA) ligands to thapsigargin, which is necessary for apoptosis, did not increase Rhod-2 fluorescence further (data not shown), consistent with the notion that the ER stress component of lipoprotein-cholesterol loading, not the PRR component, is responsible for the increase in mitochondrial calcium. In additional experiments, when Rhod-2–labeled macrophages were loaded with cholesterol for a long enough period of time to induce apoptosis, the apoptotic cells were entirely represented among the population of cells that were Rhod-2–positive (data not shown).
We next determined whether the increase in mitochondrial calcium was dependent on CaMKII. KN93, but not KN92, caused a marked decrease in Rhod-2 fluorescence in cholesterol-loaded macrophages (Figure 7A). Cells treated with the mitochondrial calcium uniporter inhibitor RU360 (45) served as a positive control for loss of mitochondrial Rhod-2 fluorescence. Consistent with the idea that these mitochondrial calcium processes were directly related to ER stress (see above), similar data were obtained using thapsigargin-treated macrophages (Figure 7B).
ER stress–induced mitochondrial calcium uptake is dependent on CaMKII. (A and B) Macrophages were incubated under control or cholesterol-loading conditions (A) or with 0.25 mM thapsigargin as the ER stressor (B) for 7 hours, in the absence or presence of 10 μM KN93, KN92, or RU360 after 1 hour pretreatment. Rhod-2 labeling and quantification were then carried out as described in Figure 5. Scale bars: 10 μm. (C) Macrophages were incubated under control or cholesterol-loading conditions for the indicated times. Cytosol-free mitochondria were isolated and immunoblotted for total CaMKII, phospho-CaMKII, and cytochrome c oxidase (Cyto ox’ase). Mitochondria (Mit), cytosol (Cyt), and ER-plasma membrane (ER PM) fractions — immunoblotted for the mitochondrial marker cytochrome c oxidase, the cytosol marker GAPDH, and the ER marker calreticulin — are also shown. (D) Macrophages were incubated under control or cholesterol-loading conditions for 12 hours with or without 10 μM RU360 after 1 hour pretreatment, and then stained with MitoTracker Red. (E) Macrophages were incubated for 20 hours with medium alone as control or with medium containing 0.25 μM thapsigargin; thapsigargin and 50 μg/ml acetyl-LDL (AcLDL); or thapsigargin, acetyl-LDL, and RU360. Apoptosis was then assayed quantified. Differing symbols indicate P < 0.01; identical symbols indicate differences that are not significant.
The role of CaMKII in mitochondrial membrane depolarization and mitochondrial calcium uptake in ER-stressed macrophages could involve a CaMKII-dependent process occurring at the mitochondrial membrane. If so, we might expect to see an increase in mitochondria-associated CaMKII upon ER stress induction. For example, activation of CaMKIIα in neurons leads to its translocation from the cytoplasm to postsynaptic membrane receptors (46). To test this idea, cytosol-free mitochondria were probed for total and phosphorylated CaMKII under control and cholesterol-loading conditions. There was a marked increase in mitochondria-associated CaMKII after 6 hours of cholesterol loading, and mitochondria also showed an increase in phospho-CaMKII under these conditions (Figure 7C; purity of the mitochondrial fraction is shown by the bottom immunoblot). These data raise the possibility that cholesterol loading, and perhaps ER stress in general, causes a translocation of CaMKII from the cytoplasm to the mitochondria.
Finally, we sought to show the predicted causal links among mitochondrial calcium uptake, Δψm, and apoptosis in the ER stress/PRR model. RU360 blocked the cholesterol-induced loss of MitoTracker Red staining (Figure 7D), indicating the role of mitochondrial calcium uptake in ER stress–induced Δψm. Most importantly, ER stress/PRR-induced apoptosis was suppressed by RU360 (Figure 7E). Thus, mitochondrial calcium uptake is induced by ER stress in a CaMKII-dependent manner, and these events are important for ER stress–induced apoptosis.
Importance of CaMKIIγ in macrophage apoptosis and Δψm in ER-stressed mice. To test the role of CaMKIIγ in macrophage apoptosis in vivo, we took advantage of a model of systemic ER stress in which mice are injected i.v. with tunicamycin (47). We treated WT and Camk2g–/– mice with tunicamycin, and, 24 hours later, harvested peritoneal macrophages and assayed them for CaMKIIγ protein, apoptosis, and mitochondrial membrane potential. As above, CaMKII protein was present in macrophages from WT mice but was undetectable in macrophages from Camk2g–/– mice (Figure 8A). Macrophages from the tunicamycin-treated WT mice showed a marked increase in apoptosis compared with vehicle-treated WT mice, and this increment was significantly blunted in macrophages from tunicamycin-treated Camk2g–/– mice (Figure 8B). Similarly, tunicamycin treatment of WT mice led to Δψm, which was not seen in macrophages from tunicamycin-treated Camk2g–/– mice (Figure 8C). Another experiment using i.p. tunicamycin was conducted to examine apoptosis in splenic macrophages in situ (Figure 8D). Tunicamycin led to a marked increase in apoptosis in CD68-positive macrophages, as well as other cells, in the spleen, and this effect was completely abrogated in Camk2g–/– mice. Thus, paralleling the data in vitro, CaMKIIγ plays an important role in macrophage apoptosis and Δψm induced by systemic ER stress in vivo.
Importance of CaMKIIγ in macrophage apoptosis and Δψm in ER-stressed mice. (A–C) WT and Camk2g–/– mice were injected i.v. with tunicamycin or vehicle control. Peritoneal macrophages were harvested 24 hours later and then assayed for CaMKIIγ protein by immunoblot analysis (A), for apoptosis by annexin V staining (B), or for mitochondrial membrane potential by MitoTracker Red staining (C). Scale bars: 10 μm. (D) WT and Camk2g–/– mice were injected i.p. with 1 mg/kg tunicamycin or vehicle control. The spleens were harvested 48 hours later and stained using TUNEL (apoptosis) or anti-CD68 (macrophages). Scale bar: 20 μm. Quantification of TUNEL-positive cells among CD68-positive cells from 3 mice per group is shown. Differing symbols indicate P < 0.01; identical symbols indicate differences that are not significant.
The renal tubular epithelium is highly responsive to ER stress inducers, and ER stress in these cells is associated with renal dysfunction and is a cellular pathological end point of a number of renal diseases (47, 48). To test the application of our model to the kidney and assess functional significance in vivo, we used the tunicamycin mouse model described above. Using RT-PCR, we found that the major isoform of CaMKII expressed in murine kidneys was CaMKIIγ (data not shown). Kidneys harvested from tunicamycin-treated WT mice show extensive apoptosis in renal tubular epithelium (Figure 9A), consistent with previous findings (47). Apoptosis in these cells was markedly suppressed in tunicamycin-treated Camk2g–/– mice. We next examined renal function in this model. Two measures of renal function, serum creatinine and urine albumin/creatinine ratio, were abnormal in tunicamycin-treated WT mice but were within normal range in Camk2g–/– mice (Figure 9B). These data indicate that CaMKIIγ has a more general role in ER stress–induced apoptosis and organ function in vivo.
Importance of CaMKIIγ in renal tubular epithelial cell apoptosis and renal function in ER-stressed mice. WT and Camk2g–/– mice were injected i.p. with 1 mg/kg tunicamycin or vehicle control. (A) The kidneys were harvested 48 hours later and stained using TUNEL (apoptosis) or DAPI (nuclei). Scale bar: 20 μm. Quantification of TUNEL-positive cells from 3 mice per group is shown. (B) Serum creatinine levels and urine albumin levels (normalized to urine creatinine) were determined for all groups of mice. Differing symbols indicate P < 0.01 (A) or P < 0.05 (B); identical symbols indicate differences that are not significant.