Frequent Calcium Oscillations Lead to NFAT Activation in Human Immature Dendritic Cells*

Spontaneous Ca2+ oscillations have been observed in a number of excitable and non-excitable cells, but in most cases their biological role remains elusive. In the present study we demonstrate that spontaneous Ca2+ oscillations occur in immature human monocyte-derived dendritic cells but not in dendritic cells stimulated to undergo maturation with lipopolysaccharide or other toll like-receptor agonists. We investigated the mechanism and role of spontaneous Ca2+ oscillations in immature dendritic cells and found that they are mediated by the inositol 1,4,5-trisphosphate receptor as they were blocked by pretreatment of cells with the inositol 1,4,5-trisphosphate receptor antagonist Xestospongin C and 2-aminoethoxydiphenylborate. A component of the Ca2+ signal is also due to influx from the extracellular environment and may be involved in maintaining the level of the intracellular Ca2+ stores. As to their biological role, our results indicate that they are intimately linked to the “immature” phenotype and are associated with the translocation of the transcription factor NFAT into the nucleus. In fact, once the Ca2+ oscillations are blocked with 2-aminoethoxydiphenylborate or by treating the cells with lipopolysaccharide, NFAT remains cytoplasmic. The results presented in this report provide novel insights into the physiology of monocyte-derived dendritic cells and into the mechanisms involved in maintaining the cells in the immature stage.

Spontaneous Ca 2؉ oscillations have been observed in a number of excitable and non-excitable cells, but in most cases their biological role remains elusive. In the present study we demonstrate that spontaneous Ca 2؉ oscillations occur in immature human monocyte-derived dendritic cells but not in dendritic cells stimulated to undergo maturation with lipopolysaccharide or other toll like-receptor agonists. We investigated the mechanism and role of spontaneous Ca 2؉ oscillations in immature dendritic cells and found that they are mediated by the inositol 1,4,5-trisphosphate receptor as they were blocked by pretreatment of cells with the inositol 1,4,5-trisphosphate receptor antagonist Xestospongin C and 2-aminoethoxydiphenylborate. A component of the Ca 2؉ signal is also due to influx from the extracellular environment and may be involved in maintaining the level of the intracellular Ca 2؉ stores. As to their biological role, our results indicate that they are intimately linked to the "immature" phenotype and are associated with the translocation of the transcription factor NFAT into the nucleus. In fact, once the Ca 2؉ oscillations are blocked with 2-aminoethoxydiphenylborate or by treating the cells with lipopolysaccharide, NFAT remains cytoplasmic. The results presented in this report provide novel insights into the physiology of monocyte-derived dendritic cells and into the mechanisms involved in maintaining the cells in the immature stage.
Dendritic cells (DCs) 2 are the most potent antigen presenting cells and are thought to be the initiators and modulators of the immune response (1). In general, DCs exist in two forms, immature DCs (iDC) and mature DCs. Immature DCs are extremely efficient at endocytosis; they reside in the peripheral tissues and continuously sample their environment for the presence of foreign antigens. After capturing antigens, they become activated and migrate to the lymphoid tissues and in the process lose the ability to take up new antigens, increase their surface expression of major histocompatibility complex II molecules and co-stimulatory molecules involved in antigen presentation to T cells, and reach their full maturation stage (1)(2)(3). Although generally correct, this picture is now proving to be too simple. For example, it was recently found that iDCs are also involved in induction and maintenance of T cell tolerance in peripheral tissues (4). Immature DCs, produced by culturing monocytes for 5 days in medium containing granulocyte-macrophage stimulating factor and interleukin-4 (IL-4), are phenotypically, morphologically, and functionally identical with iDCs occurring in vivo (5). Their maturation is controlled by Toll-like receptors (TLRs), one of the best characterized classes of pattern recognition receptors of mammalian species. Most mammalian species express about 10 -15 different TLRs that are encoded by a yet to be defined number of genes. Interestingly, distinct subsets of DCs express different TLRs, and their engagement results in DC maturation (6). In fact, monocyte-derived DCs can be induced to mature very efficiently by incubating them with nanogram to microgram (per ml) concentrations of lipopolysaccharide (LPS) through engagement of TLR4 receptors (7). In addition, other ligands such as the synthetic TLR7 ligand imidazoquinoline, a reagent already used as adjuvant in the treatment of viral infections and skin tumors (8 -10), can also induce maturation of iDCs in vitro. The signaling pathways leading to DC maturation are complex and involve nuclear translocation of the transcription factor NF-B as well as increases in the cytoplasmic Ca 2ϩ concentration ([Ca 2ϩ ]) (11)(12)(13)(14)(15). Ca 2ϩ is one of the most ubiquitous second messengers underlying cellular responses such as secretion, motility, proliferation, and death. Interestingly, Ca 2ϩ -sensitive transcription factors including NFAT and NF-B regulate the expression of Ca 2ϩ -sensitive genes including IL-2, IL-3, IL-4, tumor necrosis factor-␣, and interferon-␥ (16,17). Some cell types exhibit oscillatory changes of their cytosolic Ca 2ϩ , and these have been correlated to a variety of cellular functions. For example, in T-cells, depending on their frequency, oscillations trigger Ca 2ϩdependent activation of the transcription factors NFAT, NF-B, and c-Jun N-terminal kinase (JNK) (18). In human bone marrow-derived mesenchymal stem cells, Ca 2ϩ oscillations have been implicated in differentiation (19), in embryonic stem cell-derived primitive endodermal cells, oscillations have been implicated in the exo/endocytotic vesicle shuttle (20), and in human astrocytoma cells Ca 2ϩ oscillations have been implicated in cell migration (21). Ca 2ϩ signaling is also known to be involved in the regulation of immune cell function, and its importance is emphasized by the fact that most immune cells including DCs express several classes of Ca 2ϩ channels on their plasma membrane (22) as well as intracellular Ca 2ϩ channels belonging to the InsP 3 R and ryanodine receptor family (23)(24)(25)(26)(27)(28). In this context it is worth mentioning that the involvement of Ca 2ϩ signaling events in DC maturation has been postulated for a number of years (14,15), and we recently demonstrated that ryanodine receptor 1-mediated Ca 2ϩ signals can act synergistically with signals generated via Toll-like receptors driving DC maturation (26,27).
In the present report we show that spontaneous Ca 2ϩ oscillations occur in iDCs. These oscillations occur only in iDCs and are lost during the maturation process, and their abrogation leads to the cytoplasmic localization of endogenous NFAT. The results of this study offer additional insights into some of the signaling processes controlling maturation of DCs.

MATERIALS AND METHODS
Generation of Dendritic Cells-iDCs were generated from human peripheral blood mononuclear cells as previously described (29). Briefly, monocytes were purified by positive sorting using anti-CD14-conjugated magnetic microbeads (Miltenyi Biotech, Bergisch Gladbach, Germany). The recovered cells (95-98% purity) were cultured for 5 days at 3-4 ϫ 10 5 /ml in differentiation medium containing RPMI with 10% fetal calf serum, glutamine, nonessential amino acids, and antibiotics (all from Invitrogen) supplemented with 50 ng/ml granulocyte-macrophage stimulating factor (Laboratory Pablo Cassarà, Buenos Aires, Argentina) and 1000 units/ml IL-4 (a gift from A. Lanzavecchia, Institute for Research in Biomedicine, Bellinzona, Switzerland). Maturation was induced by the addition of LPS 1 g/ml (from Salmonella abortus equi, Sigma) to the culture medium. In some experiments DC maturation was induced by the addition of the synthetic TLR7 agonist, imidazoquinoline (3M-001) (final concentration 3 M), that was kindly provided by 3M Pharmaceuticals (St. Paul, MN).
Single Cell Intracellular Ca 2ϩ Measurements-Ca 2ϩ measurements were performed on DCs loaded with fast Ca 2ϩ indicator fluo-4 (Invitrogen; 5 M final concentration). In some experiments cells were incubated with 100 M 2-aminoethoxydiphenylborate (2-APB) (Calbiochem), 1 M Xestospongin C (Calbiochem), or 2 M thapsigargin with 0.5 mM EGTA during the loading procedure. After loading, cells were rinsed once, resuspended in Krebs-Ringer medium, and allowed to adhere to poly-L-lysine (1:60 dilution) (Sigma)-treated glass coverslips that were than mounted onto a 37°C thermostatted chamber. On-line epifluorescence images were acquired every 100 ms for 50 s using a Nikon Eclipse TE2000-E fluorescent microscope equipped with an oil immersion CFI Plan Apochromat 60ϫ TIRF objective (1.45 numerical aperture). Changes in fluorescence were detected by exciting at 488 nm and recording the emission at 510 nm via an electron multiplier C9100 -13 Hamamatsu CCD camera which allows fast data acquisition (maximal temporal resolution 1 frame (110 ϫ 110 pixels/8 ms). Where indicated, either 1 g/ml LPS or 2 M U73122 (Bio Mol) was added during the measurements. To investigate the dynamics of Ca 2ϩ influx, we measured fluorescent changes in the TIRF mode; first we identified the focal plane at the cover-glass/cell membrane contact with a surface reflective interference contrast filter, and this focal plane was maintained throughout the recordings by means of the perfect focus system that exploits an infrared laser beam and a quadrant diode for online control of the microscope focusing motor. Image analysis was performed with the MetaMorph (Molecular Devices) software package.
Endocytosis and Quantitative Gene Expression Analysis-Endocytosis was followed by incubating DCs in RPMI medium containing 0.5 mg/ml fluorescein isothiocyanate (FITC)-labeled dextran (Fluka Biochemicals, Buchs, Switzerland) for 30 min at 37°C. Cells were washed twice in ice-cold phosphatebuffered saline fixed with 1% paraformaldehyde, and the number of FITC-positive cells was assessed by flow cytometry. In some experiments, before incubation with FITC-dextran, cells were treated for 45 min with 100 M 2-APB or with LPS (1 g/ml) or with the TLR-7 agonist 3M-001 (3 M) for 18 h. Gene expression was quantified by real time PCR as previously described (26). Briefly, 1-2 ϫ 10 6 iDCs were incubated for 18 h with 1 M Xestospongin C, 100 M 2-APB, 3 M imidazoquinoline (3M-001), or 1 g/ml LPS. Total RNA was extracted and treated with deoxyribonuclease I (Invitrogen) to eliminate contaminant genomic DNA. After reverse transcription using 500 ng of RNA and the Moloney murine leukemia virus reverse transcriptase (Invitrogen), cDNA was amplified by quantitative real-time PCR in the ABI PrismTM7700 using the TaqMan technology. Commercially available exon-intron junction-designed primers for glyceraldehyde-3-phosphate dehydrogenase, CD83, CD80 CD86, interferon-␣, and IL23A (Applied Biosystems, Forster City, CA) were used. Gene expression was normalized using self-glyceraldehyde-3-phosphate dehydrogenase as reference (26). The data from DCs isolated from five donors were pooled and are expressed as -fold increase in gene expression compared with untreated iDCs.
Immunoblotting Analysis-The cytosolic fraction of 6 ϫ 10 6 DCs was extracted as described by Healy et al. (30). Briefly, cells were washed once and resuspended in 50 l of ice-cold buffer containing 20 mM HEPES, pH 7.5, 5 mM NaCl, and 2 mM EDTA to which 50 l of 20 mM HEPES, pH 7.5, 4 mM NaCl, 2 mM EDTA, and 0.8% Nonidet P-40 were added. Cells were incubated on ice for 2 min, and the nuclear and membrane fractions were removed by centrifugation (600 ϫ g, 10 min, 4°C). Laemmli loading buffer (10% glycerol, 1% ␤-mercaptoethanol, 2% SDS, 65 mM Tris-HCl, pH 6.8) was added to the supernatant (cytosolic fraction) which was boiled for 5 min and then loaded onto a 7.5% SDS-polyacrylamide gel. Proteins were transferred onto nitrocellulose, and the blots were probed with a rabbit anti-NFATc1 antibody (1:500; sc-13033, Santa Cruz Biotechnology) followed by peroxidase-conjugated protein G (1:250,000) and with mouse anti-␤ tubulin (Santa Cruz sc-5274) followed by peroxidase-conjugated antimouse IgG (1:200,000). The immunopositive bands were visualized by autoradiography using the Super Signal West Dura chemiluminescence kit from Thermo Scientific (for NFAT) and BM chemiluminescence kit from Roche Applied Science (for ␤-tubulin).
Statistical Analysis and Software Programs-Statistical analysis was performed using Student's t test for paired samples; means were considered statistically significant when the p value was Ͻ0.05. When more than two samples were compared, analysis was performed by the ANOVA test followed by the Bonferroni post hoc test. The PROC MIXED statistical analysis program (SAS 9.2) on log-transformed data were used for real-time PCR gene expression analysis from independent biological replicates. The Origin computer program (Microcal Software, Inc., Northampton, MA) was used to generate graphs and for statistical analysis. Statistical analysis of categorical data was performed using the 2 test for contingency tables with a 0.05 level of significance using R software (R development Core team 2008; R Foundation for Statistical Computing, Vienna, Austria; ISBN 3-900051-07-0) was used to perform 2 tests.

RESULTS
Immature DCs were loaded with the fast calcium indicator fluo-4 and were observed by conventional epifluorescence microscopy in the absence of added stimuli. Such cells display large rhythmic fluctuations of their cytoplasmic Ca 2ϩ (Fig. 1A) with ϳ40% of the cells exhibiting oscillations with a frequency of one peak every 12.5 s (Table 1). Interestingly, the addition of LPS (Fig. 1B) or of the TLR-7 agonist (not shown) to iDCs did not affect the high frequency oscillations nor did it cause any immediate changes in the [Ca 2ϩ ] i . On the other hand, when mature DCs (treated with 1 g/ml LPS for 18 h) were observed under identical conditions, the high frequency oscillations were no longer present (Fig. 1C). In the latter case of the 162 individual cells that were monitored,   (Fig. 1, D-F). DCs were also incubated with other pharmacological agents as shown in Table 1 (Table  1) as well as the peak fluo-4 fluorescence in iDCs (Fig. 2). These results strongly suggest that the oscillations are mainly due to InsP 3 -mediated release of Ca 2ϩ from intracellular stores, with a component (probably involved in store refilling) due to influx from the extracellular environment. The phenotype of mature DCs, on the other hand, was quite different irrespective of whether the cells had been induced to mature via TLR-4 activation (by overnight incubation with 1 g/ml LPS) or via activation of TLR-7 (by overnight incubation with 3 M imidazoquinoline (3M-001)). In fact, LPS-matured DCs did not show the high frequency oscillations but rather small and slow (1 peak/50 s) spontaneous fluctuations of their [Ca 2ϩ ] i . Interestingly, incubation with imidazoquinoline, which does not transmit a maturation signal as strong as that conveyed by LPS (see CD83 expression in Fig. 5A), resulted in DCs with an intermediate phenotype; that is, with only a small proportion of cells showing 2-8 oscillations/min whose magnitude is comparable with that exhibited by iDCs (Table 1 and Fig. 2). The slow peak Ca 2ϩ increase observed in mature DCs was reduced by more than 50% by the addition of 100 M 2-APB (Fig. 2) To directly determine whether Ca 2ϩ influx accompanies the oscillations, we examined the DCs by TIRF microscopy, which allows one to monitor changes in fluorescence occurring at the plasma membrane or within microdomains close to the plasma membrane. As shown in Fig. 3 oscillations are accompanied by [Ca 2ϩ ] i influx in iDCs. Cells were allowed to attach onto the glass coverslips, and the areas of attachment were identified with the surface reflection interference contrast filter (Fig. 3,  panel B). This focal plane was fixed using the perfect focus system, and changes in the [Ca 2ϩ ] i , which in this case represent Ca 2ϩ events occurring at or very close to the plasma membrane, were monitored (Fig. 3, panel C) (Fig. 3, panel E).
These results support the finding that oscillations of the [Ca 2ϩ ] i are a specific feature of iDC that is lost upon differentiation but convey little information as to their biological role. We hypothesized that oscillations may be implicated in maintaining the immature phenotype by acting on transcription factors, in particular on the Ca 2ϩ -sensitive transcription factor NFAT. To dissect the intracellular pathways directly downstream of the spontaneous Ca 2ϩ oscillations, we followed the intracellular localization of endogenous NFAT in oscillating iDCs or in DCs in which oscillations had been inhibited by 2-APB and in mature DCs. The cytosolic fraction of DCs was obtained from untreated iDCs, iDCs treated for 15 and 45 min with 2-APB, LPS-matured DCs, and iDCs treated with cyclosporine, a drug that reduces the nuclear translocation of NFAT by inhibiting the Ca 2ϩ -dependent phosphatase calcineurin. Fig.  4A shows a representative Western blot and Fig. 4B shows a bar graph of the intensities of the immunopositive bands of the cytosolic content of NFATc1. LPS-matured DCs, which lack the high frequency Ca 2ϩ oscillations, show the highest level of cytoplasmic expression of NFAT. Similarly, its cytoplasmic level is high in cyclosporine-treated iDCs but is significantly reduced in the cytoplasm of untreated iDCs. Treatment of the latter cells with 2-APB induced the cytoplasmic localization of NFATc1. Fig. 4C shows the subcellular localization of NFATc1 by immunofluorescence; indeed, in iDCs a number of cells exhibit nuclear distribution of NFAT (arrows), whereas iDCs treated with cyclosporine or in mature DCs the fluorescence is distributed throughout the cytoplasm. These results indicate that most of the transcription factor NFAT is targeted to the nucleus in oscillating iDCs but that abrogation of Ca 2ϩ oscillations with 2-APB results in the preservation of NFATc1 within the cytoplasm. To determine whether this was specifically related to the transcription factor NFAT or a general effect, we also followed the subcellular distribution of p65 (RelA), a component of the NF-B transcription complex (NF-B1ϩRelAϩIkB) detectable in the cytoplasm of iDCs that translocates to the nucleus upon DC maturation (12,13,26). As shown in Fig. 4D, in LPS-matured DCs NF-B is translocated to the nucleus, whereas in iDCs it shows a cytoplasmic distribution. Blocking high frequency oscillations with 2-APB does not result in the nuclear translocation of NF-B. Thus, the simple abrogation of spontaneous Ca 2ϩ oscillations is not sufficient to stimulate the cells to undergo maturation, whereas the oscillations appear to regulate nuclear targeting of NFAT and may be intimately linked to the immature phenotype. The latter hypothesis was tested by following the effect of abolishing the high frequency oscillations on the transcription of several genes characteristic of mature DCs. As shown in Fig. 5A, iDCs exhibit low transcription levels of CD80, CD86, CD83, interferon-␣, and IL23A, genes that are characteristically transcribed in mature DCs (1,26,31). Inhibition of high frequency Ca 2ϩ oscillations with Xestospongin C or 2-APB caused a significant (2-20-fold) increase in their levels of expression.
Finally we studied whether the high frequency oscillations are linked to endocytosis, an essential phenotypic characteristic of iDCs (2, 3), by comparing the capacity of iDCs, 2-APB- Experiments were performed on cells isolated from at least four different donors. **, statistical analysis was performed using the ANOVA test followed by the Bonferroni post hoc test p Ͻ 0.0002. treated iDCs, and mature DCs to endocytose FITC-labeled dextran. Fig. 5B shows that although 2-APB reduces the percentage of FITC-positive cells by 40%, thus significantly reducing the endocytic activity of iDCs, it does not result in a loss of endocytosis comparable with that seen in mature DCs (loss of ϳ80%). These results strongly suggest that abolishing the Ca 2ϩ oscillations generates a signal(s) required for DC maturation.

DISCUSSION
Spontaneous Ca 2ϩ oscillations, which are rhythmic changes in [Ca 2ϩ ] i in the absence of stimulation, have been reported in certain types of excitable and non-excitable cells such as mesenchymal stem cells, endodermal cells, human astrocytoma cells, astrocytes, pancreatic acinar cells, cardiac myocytes, oocytes, and fibroblasts (19 -21, 32-35), although their intracellular mediators and biological role(s) and the functional consequence of their inhibition have in many cases not been elucidated. In the present study we show that spontaneous Ca 2ϩ oscillations also occur in human DCs and that these Ca 2ϩ events are an exclusive characteristic of cells in the immature stage. In fact, the addition of LPS as well as maturation triggered by other stimuli leads to the loss of the spontaneous high frequency Ca 2ϩ transients. A similar finding concerning the loss of spontaneous Ca 2ϩ oscillations induced by differentiation was reported in human mesenchymal stem cells upon differentiation into adipocytes (19) and in osteogenic cells upon differentiation into osteoblasts (36,37). Interestingly, in stem cells Ca 2ϩ oscillations occur during the G 1 to S transition, suggesting their involvement in cell cycle progression (38,39). On the other hand, in vitro monocyte-derived DCs do not actively proliferate but, rather, acquire the biochemical and immunological characteristics of naturally occurring iDCs (5) indicating that in these cells the oscillations are probably not involved in cell division.
In immature dendritic cells, intracellular Ca 2ϩ stores and InsP 3 are intimately connected with the high frequency oscillations, as they were completely abolished by depleting stores with the Ca 2ϩ -ATPase inhibitor thapsigargin (2 M) in the presence of EGTA (0.5 mM). The lack of high frequency Ca 2ϩ oscillations in mature LPS-treated DCs could not be explained by different levels of expression of functional InsP 3 R as mature DCs respond to ATP an InsP 3 -mobilizing agonist (23) with a Ca 2ϩ transient of comparable magnitude in the mature and immature stage (results not shown). As to the intracellular mediator(s) of the Ca 2ϩ oscillations, U73122, an inhibitor of phospholipase C (40), completely blocked Ca 2ϩ transients, whereas both 2-APB, a rather unspecific inhibitor of the InsP 3 R also inhibiting Ca 2ϩ entry (41,42), and Xestospongin C, an inhibitor of InsP 3 R-mediated Ca 2ϩ release (43), significantly decreased the frequency and magnitude of these events. The differences in response to these compounds could be explained by the contribution of Ca 2ϩ influx to the maintenance of the Ca 2ϩ oscillations. To further address this question, we performed intracellular Ca 2ϩ measurements in medium containing 2 mM Ca 2ϩ or in the presence of 100 M La 3ϩ to block Ca 2ϩ entry. Under these conditions Ca 2ϩ fluctuations were still present, but there was a reduction in the percentage of cells showing high frequency (Ͼ4 transients/50 s) Ca 2ϩ transients. This result together with the TIRF Ca 2ϩ measurements support the hypothesis that Ca 2ϩ influx is necessary to maintain the high frequency Ca 2ϩ oscillations characteristic of immature dendritic cells through a refilling mechanism.
The most intriguing question arising from the observation that monocyte-derived dendritic cells in the immature stage show frequent Ca 2ϩ oscillations concerns the biological role(s) of the oscillations. In macrophages, Ca 2ϩ oscillations have been reported to accompany phagocytosis, suggesting a relationship between Ca 2ϩ oscillations and uptake of foreign particles (44,45). In vivo, immature DCs continuously sample their environment for foreign antigens, and indeed one of the main functions of iDCs is antigen capture by endocytosis. We originally In each lane the proteins present in the cytoplasmic extract of 6 ϫ 10 6 cells was separated on 7.5% SDS-polyacrylamide gel and blotted onto nitrocellulose. The blot was cut into two; the upper portion (Ͼ60 kDa) was incubated with rabbit anti-NFATc1 followed by peroxidase-conjugated anti-rabbit IgG. The lower portion was used as a control for protein loading and developed with ␤-tubulin.  , where data from four donors were pooled, and CD83 (DCϩ2-APB), where data from three donors were pooled. Statistical analysis was performed using the PROC MIXED SAS 9.2 statistical analysis program. *, p Ͻ 0.0001; **, p Ͻ 0.00025; ***, p Ͻ 0.001. B, endocytosis of FITC-labeled dextran is shown. Cells treated as described for panel A were plated in 12-well plate and incubated at 37°C for 30 min with 0.5 mg/ml of FITC-labeled dextran. Negative controls were also incubated with FITC-labeled dextran but kept for 30 min at 4°C. Cells were washed 2 times with ice-cold phosphate-buffered saline and fixed with 1% paraformaldehyde, and the % of FITC-positive (ϩve) cells was assessed by flow cytometry. Bar graphs represent the mean (ϮS.E.) % of fluorescent cells; fluorescent value obtained for iDC was considered 100%. Results from 3-8 experiments from 3-8 different donors were pooled and averaged. Statistical analysis was performed using the ANOVA test followed by the Bonferroni post hoc test. *, p Ͻ 0.018; **, p Ͻ 0.0003. MAY 21, 2010 • VOLUME 285 • NUMBER 21 hypothesized that the high frequency Ca 2ϩ oscillations may be involved in activation of endocytosis, and blocking Ca 2ϩ oscillations with 2-APB resulted in a significant but partial decrease of FITC-dextran endocytosis, suggesting that the high frequency oscillations may not be essential for endocytosis as reported in embryonic stem cell-derived primitive endodermal cells (20). Alternatively, the inhibitory effect of 2-APB may reflect the fact that endocytosis is a Ca 2ϩ -dependent event requiring InsP 3 R activation and/or Ca 2ϩ influx (46,47). On the other hand, the involvement of Ca 2ϩ signaling in maturation had been previously documented (26,28), and it was shown that DC maturation is enhanced by activation of ryanodine receptor-mediated Ca 2ϩ release. The results obtained by real time PCR strongly suggest that pharmacological interventions, which decrease the high frequency oscillations, activate signals that are necessary but not sufficient to induce full DC maturation.

Immature Dendritic Cells Exhibit Spontaneous Ca 2؉ Oscillations
We next turned our attention to Ca 2ϩ -sensitive transcription factors as Ca 2ϩ oscillations have been shown to promote the expression of specific genes in other cell systems (39,48). We focused our attention on NFAT, a calcineurin-dependent transcription factor, as early work demonstrated that NFAT has the remarkable capacity to sense dynamic changes in the [Ca 2ϩ ] i and is especially tuned to detect high frequent Ca 2ϩ oscillations occurring within cells (48,49). In fact, high frequency oscillations have been shown to activate NFAT by keeping the transcription factor in the nucleus at high enough levels to bind to enhancer sites long enough to allow initiation of transcription. Because in our case only iDCs possess these high frequency Ca 2ϩ fluctuations, NFAT should be active and translocated into the nucleus only in iDCs and not in LPS-matured DCs. Western blot analysis of endogenous NFAT indeed showed that the cytosolic fraction of iDCs contains considerable less immunopositive band compared with that present in mature DCs; furthermore, by shutting off the Ca 2ϩ oscillations with 2-APB, NFAT is retained in the cytoplasm. As opposed to what was observed for NFAT, the transcription factor NF-B is activated and translocated into the nucleus in LPS-matured DCs but not in iDCs nor in 2-APB-treated DCs. Thus, simply blocking the high frequency Ca 2ϩ oscillations or blocking nuclear translocation of NFAT is not sufficient to induce either nuclear translocation of NF-B or DC maturation.
Altogether these results indicate that the high frequency Ca 2ϩ oscillations depend on the maturation stage of DCs, and we suggest that they act as "frequency encoding" (as opposed to amplitude encoding) signals, whereby through the activation of NFAT, DCs maintain their immature phenotype. Our data do not support recent results showing that LPS induces a transient increase in [Ca 2ϩ ] i in DCs (50 -52). We directly tested whether the addition of LPS (1 g/ml) to iDCs causes an increase in the cytoplasmic [Ca 2ϩ ] i but failed to obtain any response. Similarly, no changes in the [Ca 2ϩ ] i on plasma membrane microdomains after the addition of LPS were observed by TIRF microscopy (data not shown). The differences between our results and those presented in Refs. 50 -52 are most likely due to the different experimental models that were used; that is, human monocyte-derived DCs in this study versus mouse bone marrow-derived DCs. In fact, as opposed to mouse DCs, immature human DCs express very low levels of CD14, and thus, the CD14-dependent Ca 2ϩ signaling pathways may be absent in our system. Our possibility of using the TIRF microscope has enabled us to directly monitor membrane-associated events, and our results together with those of Matzner et al. (51) argue against a major role of Ca 2ϩ influx in LPS-mediated Ca 2ϩ signaling.
In conclusion, we report that human monocyte-derived iDCs exhibit spontaneous [Ca 2ϩ ] i oscillations that are linked to InsP 3 R activation and to, a lesser extent, to Ca 2ϩ influx. These high frequency events are lost during maturation and appear to be an endogenous characteristic of the immature phenotype, possibly activating nuclear translocation of NFAT and, thus, enhancing the transcription of genes involved in maintaining the cells immature. The results of the present investigation are important because they point out novel aspects of intracellular signaling in human DC and may open new areas of research that could be developed in the future to help patients requiring modulation of their immune response.