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Role of Sphingosine 1-Phosphate in the Pathogenesis of Sjögren’s Syndrome¹

Masahiro Sekiguchi^*, Tsuyoshi Iwasaki^2,*, Masayasu Kitano^*, Hideki Kuno^*, Naoaki Hashimoto^*, Yutaka Kawahito, Masayuki Azuma, Timothy Hla and Hajime Sano^*

^* Division of Rheumatology and Clinical Immunology, Department of Internal Medicine, Hyogo College of Medicine, Hyogo, Japan; Inflammation and Immunology, Graduate School of Medical Science, Kyoto Prefectural University of Medicine, Kyoto, Japan; Department of Oral and Maxillofacial Surgery 2, Tokushima University School of Density, Tokushima, Japan; and Center for Vascular Biology, Department of Cell Biology, University of Connecticut Health Center, Farmington, CT 06030

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
Primary Sjögren’s syndrome (SS) is an autoimmune disease characterized by inflammatory mononuclear cell infiltration and destruction of epithelial cells of lacrimal and salivary glands. Sphingosine 1-phosphate (S1P) and signaling through its receptor S1P₁ have been implicated in many critical cellular events including inflammation, cancer, and angiogenesis. This study was undertaken to examine the role of S1P₁ signaling in the pathogenesis of primary SS. S1P₁ and sphingosine kinase 1, which converts sphingosine to S1P, were detected in the cytoplasm of inflammatory mononuclear cells, vascular endothelial cells, and epithelial cells in all labial salivary glands by immunohistochemistry. The expression of S1P₁ in inflammatory mononuclear cells was enhanced in advanced stages of primary SS. S1P enhanced proliferation and IFN- production by CD4⁺ T cells. The enhancing effect of S1P on IFN- production by CD4⁺ T cells was stronger in patients with primary SS than in healthy controls. S1P also enhanced Fas expression and Fas-mediated caspase-3 induction in salivary gland epithelial cells. IL-6 expression was detected in the cytoplasm of inflammatory mononuclear cells and ductal epithelial cells and was enhanced in advanced stages of primary SS. Furthermore, both IFN- and S1P augmented IL-6 secretion by salivary gland epithelial cells. These effects of S1P were inhibited by pretreatment of pertussis toxin. Our data reveal that S1P₁ signaling may modulate the autoimmune phenotype of primary SS by the action of immune as well as epithelial cells.

	Introduction

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Primary Sjögren’s syndrome (SS)³ is an autoimmune disease characterized by inflammatory mononuclear cell infiltration and destruction of acinar and ductal epithelial cells of lacrimal and salivary glands. The inflammatory mononuclear cell infiltration in primary SS is mainly represented by CD4⁺ T cells (1). The inflammatory mononuclear infiltrates within the inflamed glands often contain germinal center-like structures consisting of T and B cell aggregates with a network of proliferating lymphocytes, follicular dendritic cells, and activated endothelial cells (2). Analysis of inflamed glandular tissue from patients with primary SS also revealed a polyclonal accumulation of CD27⁺ memory B cells and CD27^high plasma cells with a diminished frequency and absolute number of peripheral CD27⁺ memory B cells (3, 4). Although analysis of expression of Th1 and Th2 cytokine mRNA levels in labial salivary glands (LSG) has generated conflicting results (5, 6, 7), IL-6 mRNA is highly expressed in patients with primary SS (8). There is also growing evidence indicating that acinar and ductal epithelial cells of salivary and lachrymal glands undergo apoptosis mediated through Fas or the perforin pathway (9). In addition, there is an increasing amount of data suggesting that the salivary gland epithelial cells are active participants in the initiation of the inflammatory process (10).

Sphingosine 1-phosphate (S1P) is one of the cell-derived lysophospholipid growth factors that signal diverse cellular functions (11). S1P is generated by metabolism of sphingomyelin with S1P levels being tightly regulated by series of enzymes including sphingosine kinase (SK) and S1P phosphatase. S1P acts as an extracellular mediator by binding to G protein-coupled receptors (GPCRs). To date, five closely related GPCRs, namely S1P₁, S1P₂, S1P₃, S1P₄, and S1P₅, have been identified as high-affinity S1P receptors (12) (see Fig. 1). S1P was defined as a novel regulator of angiogenesis and seems to be a major bioactive lysophospholipid that is released from platelets and interacts with endothelial cells through S1P₁ (13). In the immune system, S1P interacts with naive and memory T cells through S1P₁, regulating T cell development and tissue-homing patterns (14, 15). The aim of the present study was to evaluate the role of S1P₁ signaling for the pathogenesis of primary SS. The results provided in this study strongly support a significant role of S1P₁ signaling for the local immune responses in salivary glands of patients with primary SS.

View larger version (19K): [in this window] [in a new window]   FIGURE 1. Pathways of S1P metabolism. Graphic representation shows S1P is generated by metabolism of sphingomyelin with S1P levels being tightly regulated by series of enzymes including SK and S1P phosphatase. S1P acts as an extracellular mediator by binding to GPCRs and promotes cell proliferation and differentiation, whereas sphingosine and ceramide inhibit cell proliferation and stimulate apoptosis. The balance of these three important lipid-signaling molecules is critically regulated by SK1, the agonist-inducible isoform that can be activated by a variety of growth factors, cytokines and mitogens. S1P1 is one of the GPCRs of S1P, which promotes angiogenesis and the recruitment of lymphocytes.

	Materials and Methods

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Peripheral bloods for CD4⁺ T cell isolations were obtained from six healthy volunteers (four women and two men) with a mean age of 39.5 years (range 31–55 years) and five patients with primary SS (four women and one man) with a mean age of 43.5 years (range 33–67 years). LSG biopsy samples were obtained from 16 patients with primary SS (15 women and 1 man) with a mean age of 53.5 years (range 23–79 years). The healthy controls were subjected who had experienced subjective symptoms of oral dryness, but met none of the objective criteria for a diagnosis of primary SS. Informed consent was obtained from all subjects before CD4⁺ T cells sampling and LSG biopsy were performed, and the institutional medical ethics committee approved the study protocol. All patients fulfilled the American-European Consensus Group criteria for a diagnosis of primary SS (16). Grading of LSG biopsies was performed based on size and degree of lymphoid organization of the infiltrates (17). Briefly, lymphocytes and plasma cells per 4 mm² were counted. Cellular aggregate with 50 or more lymphocytes, histiocytes, and plasma cells were defined as focus. Grade 1 is characterized by slight infiltration. Grade 2 displayed moderate infiltrate or less than one focus per 4 mm³. Grade 3 displayed one focus per 4 mm³. Grade 4 displayed more than one focus per 4 mm³.

Immunohistochemistry for S1P₁ SK1, CD4, IFN-, and IL-6 expression in LSG

LSG tissue specimens were preserved in 10% formalin, embedded in paraffin, and serially sectioned onto microscope slides at a thickness of 4 µm. Immunostaining was performed with peroxidase labeling techniques (18). All procedures were performed at room temperature. Tissue sections were deparaffinized, and endogenous peroxidase activity was blocked by incubation in 0.3% peroxide in methanol for 45 min. S1P₁ staining was performed as follows. The sections were preincubated with 1% FBS in PBS for 60 min followed by incubation overnight with either the primary Ab against human S1P₁ (purified IgY from a chicken immunized with human S1P₁) or preimmune chicken serum (1/200 dilution in PBS) (19). Sections were then washed in PBS and incubated with HRP-conjugated anti-chicken IgY (1/200 dilution in PBS) for 60 min. The sections were further washed with PBS, and the color was developed by immersing the sections in a solution of 0.05% (w/v) 3,3-diaminobenzidine tetrahydrochloride (Sigma-Aldrich) and 0.01% hydrogen peroxide in 0.05 M Tris (pH 7.4) for 3 min. The sections were counterstained with Mayer’s hematoxylin solution (Wako Pure Chemicals). SK1, CD4, IFN-, or IL-6 staining was performed with the Vectastain ABC kit (Vector Laboratories), according to the manufacturer’s suggested protocol using the primary Ab against human SK1 (1/250 dilution in PBS) (purified polyclonal Ab from a rabbit immunized with human SK1) (20), the primary Ab against human CD4 (1/20 dilution in PBS) (NovoCastra Laboratories) (21), the primary Ab against human IFN- (1/40 dilution in PBS) (R&D Systems) (22), or the primary Ab against human IL-6 (1/50 dilution in PBS) (Santa Cruz Biotechnology), respectively (23). Positive staining was indicated by a brownish deposit, and background staining was purple.

Cell line

NS-SV-DC cell line (24) is immortalized normal salivary gland ductal cells established by transfection with SV40, cultured in serum-free keratinocyte medium (Invitrogen Life Technologies). HUVECs were purchased from Cambrex Bio Science and were cultured in EGM Bulletkit (Takara Shuzo).

RNA preparation and analysis of S1P₁, Fas mRNA

Preparations of total RNA from CD4⁺ T cells and NS-SV-DC cells were performed using Isogen (Nippon Gene) according to the manufacturer’s protocol. Reverse transcription and cDNA amplification were performed by the TaKaRa RNA PCR kit (Takara) (25). The following primers were used for the RT-PCR analysis: human S1P₁ (429 bp product), sense 5'-TATCAGCGCGGACAAGGAGAACAG-3' and antisense 5'-ATAGGCAGGCCACCCAGGATGAG-3'; human Fas (500 bp product), sense 5'-TTCGGAGGATTGCTCAACA-3' and antisense 5'-GGTGAGTGTGCATTCCTTG-3'; and GAPDH (246 bp product), sense 5'-GATGACATCAAGAAGGTGGTGAA-3' and antisense 5'-GTCTTACTCCTTGGAGGCCAT-GT-3'. Amplification was performed at 94°C for 1 min, 62°C for 1 min, and 72°C for 1 min in a DNA thermal cycler (PerkinElmer Cetus Instruments) for 26, 29, and 32 cycles to ensure linearity. PCR products were electrophoresed on a 2% agarose gel and visualized by ethidium bromide staining. The S1P₁ and Fas PCR products were normalized in relation to the GAPDH internal control.

CD4⁺ T cell isolation

CD4⁺ T cells were isolated from peripheral blood from healthy volunteers and from patients with primary SS. Briefly, mononuclear cells were isolated from peripheral blood by Ficoll-Paque density gradient centrifugation. Mononuclear cells (1 x 10⁷) were labeled with biotin-conjugated anti-CD4 mAb and magnetic anti-biotin microbeads according to the manufacturer’s protocol (CD4⁺ T cell isolation kit II; Miltenyi Biotec) and CD4⁺ T cells were separated using miniMACS separator (Miltenyi Biotec). Purity of the CD4⁺ T cell population was >95%.

Cell proliferation studies

The 96-well plates were coated overnight at 4°C with 0.5 µg/ml anti-CD3 mAb and washed three times with PBS. CD4⁺ T cells (2 x 10⁴/100 µl/well) and 30 Gy-irradiated autologous PBMC (1 x 10⁵/100 µl/well) were cultured in serum-free medium (AIM-V; Invitrogen Life Technologies) without or with S1P (0.01–0.5 µM) in anti-CD3 mAb-coated 96-well plates. After 3 days of culture, 1 µCi/well [³H]thymidine (Amersham Biosciences) was added to each well, and 16 h later incorporation was assessed.

Measurement of IFN- secretion

The 24-well plates were coated overnight at 4°C with 0.5 µg/ml anti-CD3 mAb and washed three times with PBS. CD4⁺ T cells (2 x 10⁵/ml/well) and 30 Gy-irradiated autologous PBMC (1 x 10⁶/ml/well) were cultured in serum-free medium (AIM-V; Invitrogen Life Technologies) without or with S1P (0.01–0.5 µM) in anti-CD3 mAb-coated 24-well plates. After 48 h of culture, the supernatants were collected, and IFN- concentrations in the supernatants were measured by ELISA.

Measurement of IL-6 secretion

NS-SV-DC cells (5 x 10⁵/ml/well) were cultured in the absence or presence of S1P (0.01–0.5 µM) or IFN- (0.2 µg/ml) in serum-free keratinocyte medium (Life Technologies). After 48 h of culture, the supernatants were collected and IL-6 concentrations in the supernatants were measured by ELISA.

IFN- and IL-6 ELISA

The concentrations of IFN- and IL-6 in the culture supernatants were measured by ELISA using Quantikine ELISA kit according to the manufacturer’s protocol (R&D Systems).

Measurement of caspase-3 activity

Caspase-3 activity was measured using Caspase-3 Colorimetric Assay (R&D Systems) according to manufacturer’s protocol. NS-SV-DC cells (1 x 10⁶) were cultured in serum-free keratinocyte medium in the absence or presence of S1P (0.01–0.5 µM) or IFN- (0.2 µg/ml) in 6-well plates. After 72 h of culture, anti-Fas mAb (100 ng/ml; Medical Biological Laboratories) was added and cultured an additional 6 h, and the cells were collected by centrifugation. The cell lysates were transferred into 96-well plate and mixed with buffer and caspase-3 colorimetric substrate (DEVD-pNA). After 2 h of incubation at 37°C, caspase-3 activity was determined by a microplate spectrophotometer (SpectraMax, Molecular Devices).

Detection of apoptosis

DNA chromosome morphology was assessed using HOECHST staining. NS-SV-DC cells treated with S1P were labeled with 8 mg/ml HOECHST 33342 (Sigma-Aldrich) for 10 min and the cells were examined by fluorescence microscopy.

Measurement of the effect of pertussis toxin (PTX) on S1P-enhanced IFN- production by CD4⁺ T cells and Fas mRNA expression by NS-SV-DC cells

CD4⁺ T cells were preincubated for 24 h in the presence of 100 ng/ml PTX (Sigma-Aldrich). After rigorous washing, cells were stimulated with anti-CD3 mAb (0.5 µg/ml) in the presence of S1P. After 48 h of culture, IFN- concentrations in the culture supernatants were measured. PTX-pretreated NS-SV-DC cells were treated with S1P or IFN- (0.2 µg/ml) for 6 h, and Fas mRNA expression in NS-SV-DC cells was analyzed by RT-PCR.

Statistical analysis

Results are expressed as mean ± SD. Student’s t test was used to compare individual treatments with their respective control values. A value for p < 0.05 was considered statistically significant.

	Results

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Tissue distribution of SK1 and S1P₁ expression in salivary glands from patients with primary SS

S1P promotes cell proliferation and survival, whereas sphingosine and ceramide inhibit cell proliferation and stimulate apoptosis. The balance of these three important lipid-signaling molecules is critically regulated by SK, which converts sphingosine to S1P by phosphorylating sphingosine (Fig. 1). SK1, the agonist-inducible isoform that can be activated by a variety of growth factors, cytokines, and mitogens, has been implicated in cell transformation and tumor growth (26, 27, 28). S1P₁ is one of the GPCRs of S1P, which promotes angiogenesis and recruitment of lymphocytes (13, 14, 15). To study the role of S1P-S1P₁ interactions in the pathogenesis of primary SS, we examined the expression and localization of SK1 and S1P₁ in LSG from patients with primary SS by immunohistochemistry. The immunoreactivity of both SK1 and S1P₁ exhibited a similar cellular distribution, as both SK1 and S1P₁ were expressed within cytoplasm of inflammatory mononuclear cells, vascular endothelial cells, and salivary gland epithelial cells in LSG biopsy specimens (Fig. 2). We next extended this approach to various stages of sialoadenitis and examined the extent and intensity of both SK1 and S1P₁ immunostaining. Fig. 3 shows representative SK1 and S1P₁ immunohistochemistry in LSG biopsy specimens. Although SK1 staining intensity was not different between grade 1 and grade 4 LSG biopsy specimens, S1P₁ staining in inflammatory mononuclear cells was significantly more extensive in the grade 4 LSG biopsy specimens than in the grade 1 LSG biopsy specimens (Fig. 3, E and G). These results indicate that S1P-S1P₁ interactions occur in salivary glands from patients with primary SS.

View larger version (83K): [in this window] [in a new window]   FIGURE 2. Patterns of S1P1 and SK1 expression in grade 4 LSG biopsy specimens from patients with primary SS. Immunohistochemistry for S1P1 (B and E) and for SK1 (C and F) was performed on 4-µm thick sections of grade 4 LSG biopsy specimens from patients with primary SS. Control staining with preimmune chicken serum (A and D) was also performed. The same biopsy sections were used to analyze both SK1 and S1P1. Both SK1 and S1P1 were expressed within cytoplasm of inflammatory mononuclear cells, vascular endothelial cells, and salivary gland epithelial cells in LSG biopsy specimens. Original magnification, x200, with insets, x1000 (B and C). Grade 4 displayed more than one focus per 4 mm3. Cellular aggregate with 50 or more lymphocytes, histiocytes, and plasma cells was defined as one focus. BV, Blood vessel; EP, epithelial cell; MN, mononuclear cell.

View larger version (94K): [in this window] [in a new window]   FIGURE 3. Characterization of SK1 and S1P1 expression and histologic grading in LSG biopsy specimens from patients with primary SS. Immunohistochemistry for SK1 (B, D, and F) and for S1P1 (C, E, and G) was performed on 4-µm-thick sections of control (B and C), grade 1 (D and E) and grade 4 (F and G) LSG biopsy specimens. Control staining with preimmune chicken serum (A) was also performed. The same biopsy sections were used to analyze both SK1 and S1P1. Original magnification, x400, with insets, x1000. A trend toward an increase of S1P1 expression in inflammatory mononuclear cells with increasing histologic grading (E and G) is shown. Grade 1 is characterized by slight infiltration and grade 4 displayed more than one focus per 4 mm3. Cellular aggregate with 50 or more lymphocytes, histiocytes, and plasma cells was defined as one focus. EP, Epithelial cell; MN, mononuclear cell.

Inflammatory mononuclear cells in primary SS are mainly represented by CD4⁺ T cells (1). Because S1P₁ was significantly overexpressed in infiltrating inflammatory mononuclear cells in the salivary glands from advanced stages of primary SS (Fig. 3, E and G), we investigated the effect of S1P on CD4⁺ T cell functions. First, we examined whether CD4⁺ T cells from peripheral blood expressed S1P₁ using RT-PCR analysis. As shown in Fig. 4A, magnetically purified CD4⁺ T cells from both healthy volunteers and patients with primary SS expressed S1P₁ (Fig. 4A). Next, we examined the effect of S1P on CD4⁺ T cell proliferation. The proliferation of CD4⁺ T cells was not affected by S1P alone (data not shown). However, when CD4⁺ T cells were stimulated with plate-bound anti-CD3 mAb, addition of S1P (0.01–0.5 µM) enhanced the proliferation of CD4⁺ T cells (Fig. 4B). We also examined whether S1P had a role in the secretion of IFN- by CD4⁺ T cells. Interestingly, S1P, at the same concentrations used in the proliferation assay (0.01–0.5 µM), enhanced IFN- secretion by CD4⁺ T cells (Fig. 4C). We compared enhancing effects of S1P on proliferation and IFN- secretion by CD4⁺ T cells from healthy controls and from patients with primary SS. The effect of S1P to enhance IFN- secretion by CD4⁺ T cells was stronger in patients with primary SS than in healthy controls, although the effect of S1P to enhance proliferation by CD4⁺ T cells was not different between these two groups (Fig. 5). To characterize the IFN--secreting CD4⁺ T cells present in LSG tissue, serial sectioned LSG biopsy samples from patients with primary SS were labeled with anti-CD4 or anti-IFN- Abs. Fig. 6 shows a representative section from LSG tissue. The majority of CD4⁺ T cells accumulated at LSG stained positive for IFN- (Fig. 6). These results indicate that S1P enhances TCR-stimulated CD4⁺ T cell proliferation and IFN- secretion and that the effect of S1P to enhance IFN- secretion by CD4⁺ T cells is augmented in patients with primary SS.

View larger version (26K): [in this window] [in a new window]   FIGURE 4. S1P1 expression and S1P responses by CD4+ T cells. A, RT-PCR analysis of S1P1 mRNA levels in peripheral blood CD4+ T cells. RNA isolated from magnetically sorted peripheral blood CD4+ T cells from healthy volunteers (C1–C3) and from patients with primary SS (P1–P3) was reverse transcribed to cDNA and amplified by RT-PCR. Primers for S1P1 or GAPDH generated the expected 429-bp or 246-bp band, respectively. HUVECs (H) were used as a positive control. B, Effect of S1P on CD4+ T cell proliferation. Magnetically sorted peripheral blood CD4+ T cells (2 x 104/200 µl/well) and irradiated (30 Gy) autologous PBMC (1 x 105/200 µl/well) were incubated with plate-bound anti-CD3 mAb (0.5 µg/ml) in the absence (–) or presence (+) of 0.01–0.5 µM S1P. After 72 h of culture, [3H]thymidine was added for an additional 16 h and incorporation was assessed. Data represent mean ± SD from five independent experiments. *, p < 0.05. C, Effect of S1P on IFN- secretion by CD4+ T cells. Magnetically sorted peripheral blood CD4+ T cells (2 x 105/ml/well) and irradiated (30 Gy) autologous PBMC (1 x 106/ml/well) were incubated with plate-bound anti-CD3 mAb (0.5 µg/ml) in the absence (–) or presence (+) of 0.01–0.5 µM S1P. After 48 h culture, culture supernatants were collected, and IFN- levels were measured by ELISA. Data represent mean ± SD from five independent experiments. *, p < 0.05.

View larger version (12K): [in this window] [in a new window]   FIGURE 5. S1P responses by CD4+ T cells from patients with primary SS () and healthy controls (). A, Effect of S1P on CD4+ T cell proliferation. Magnetically sorted peripheral blood CD4+ T cells (2 x 104/200 µl/well) and irradiated (30 Gy) autologous PBMC (1 x 105/200 µl/well) were incubated with plate-bound anti-CD3 mAb (0.5 µg/ml) in the absence or presence of 0.01 or 0.1 µM S1P. After 72 h of culture, [3H]thymidine was added for an additional 16 h and incorporation was assessed. Percentage of increase of anti-CD3 mAb-induced proliferation was calculated according to the following formula: (anti-CD3 mAb-induced proliferation in the presence of S1P – anti-CD3 mAb-induced proliferation in the absence of S1P)/(anti-CD3 mAb-induced proliferation in the absence of S1P) x 100. Data represent mean ± SD of percentage of increase in proliferation obtained from five independent experiments. NS, Not significant. B, Effect of S1P on IFN- secretion by CD4+ T cells. Magnetically sorted peripheral blood CD4+ T cells (2 x 105/ml/well) and irradiated (30 Gy) autologous PBMC (1 x 106/ml/well) were incubated with plate-bound anti-CD3 mAb (0.5 µg/ml) in the absence or presence of 0.01 or 0.1 µM S1P. After 48 h culture, culture supernatants were collected and IFN- levels were measured by ELISA. Percentage increase of anti-CD3 mAb-induced IFN- secretion was calculated according to the following formula: (anti-CD3 mAb-induced IFN- secretion in the presence of S1P – anti-CD3 mAb-induced IFN- secretion in the absence of S1P)/(anti-CD3 mAb-induced IFN- secretion in the absence of S1P) x 100. Data represent mean ± SD of percentage of increase in IFN- secretion obtained from five independent experiments. *, p < 0.05.

View larger version (114K): [in this window] [in a new window]   FIGURE 6. Characterization of IFN--secreting CD4+ T cells in LSG biopsy specimens from patients with primary SS. Immunohistochemistry for CD4 (A and C) and IFN- (B and D) was performed on 4-µm thick sections of grade 4 LSG biopsy specimens from patients with primary SS. Original magnification, x400 (A and B) and x1000 (C and D). Positive staining of cells for CD4 and IFN- was present at similar sites within the tissue. Grade 4 displayed more than one focus per 4 mm3. Cellular aggregates with 50 or more lymphocytes, histiocytes, and plasma cells were defined as one focus.

Because S1P₁ was strongly expressed in epithelial cells in the salivary glands of patients with primary SS (Figs. 2 and 3), we next examined the effect of S1P on a salivary gland ductal epithelial cell line (NS-SV-DC). Apoptosis of the ductal epithelial cells of salivary and lacrimal glands has been proposed as a possible mechanism responsible for primary SS. Apoptotic cell death may be induced by interaction between Fas on epithelial cells and Fas ligand expressed by T cells. There are in vitro findings that an unstimulated human salivary gland cell line constitutively expressed low levels of Fas, and IFN- secreted by lymphocytes may up-regulate Fas expression on epithelial cells, thus increasing their sensitivity to apoptotic death signals (29). We observed that IFN- significantly increased Fas mRNA expression in NS-SV-DC. Fas mRNA expression was also significantly increased by S1P (0.1–0.5 µM). Furthermore, S1P enhanced IFN--induced Fas mRNA expression in NS-SV-DC cells (Fig. 7A). These results indicate that both S1P and IFN- secreted by infiltrating CD4⁺ T cells increase Fas expression on salivary gland epithelial cells. The activation of caspase-3 appears to be indispensable for the apoptotic process (30). Therefore, we examined caspase-3 expression in NS-SV-DC cultured with IFN- or S1P. As shown in Fig. 7B, both IFN- and S1P (0.1–0.5 µM) significantly increased caspase-3 expression in NS-SV-DC in the presence of anti-Fas mAb (Fig. 7B). We also confirmed apoptosis of NS-SV-DC cells treated with anti-Fas mAb and S1P by HOECHST staining (data not shown). These results indicate that both IFN- and S1P induce apoptosis via Fas signaling by salivary gland epithelial cells.

View larger version (17K): [in this window] [in a new window]   FIGURE 7. Effect of S1P on Fas mRNA expression and caspase-3 activity in salivary gland epithelial cells. A, NS-SV-DC cells (1 x 106) were treated with 0.01–0.5 µM S1P without (–) or with (+) IFN- (0.2 µg/ml) for 6 h, and semiquantitative RT-PCR for the expression of Fas mRNA in NS-SV-DC cells was performed. Fas mRNA expression levels were determined by normalizing expression with respect to GAPDH mRNA expression levels. Data represent mean ± SD from three to six independent experiments. *, p < 0.05; #, p < 0.01. B, NS-SV-DC cells (1 x 106) were cultured in the presence (+) or absence (–) of S1P (0.01–0.5 µM) or IFN- (0.2 µg/ml). After 72 h of culture, anti-Fas mAb (100 ng/ml) was added and caspase-3 activity of the cell lysates was analyzed. Percentage increase of anti-Fas mAb-induced caspase-3 activity was calculated according to the following formula: (anti-Fas mAb-induced caspase-3 activity in the presence of S1P or IFN- – anti-Fas mAb-induced caspase-3 activity in the absence of S1P and IFN-)/(anti-Fas mAb-induced caspase-3 activity in the absence of S1P and IFN-) x 100. Data represent mean ± SD of percentage increase of caspase-3 activity determined from three to six independent experiments. *, p < 0.05.

IL-6 is known to be a B cell growth and differentiation factor and is generally found to be highly expressed in many autoimmune diseases (31). Although serum levels of IL-6 have generated conflicting results, analysis of tear and salivary IL-6 levels in patients with primary SS are elevated when compared with those in healthy controls (32, 33, 34). We examined IL-6 expression in the salivary glands from patients with primary SS by immunohistochemistry. IL-6 was detected in the cytoplasm of most inflammatory mononuclear cells and ductal epithelial cells. Furthermore, the extent and intensity of IL-6 expression in ductal epithelial cells correlated with mononuclear cell infiltration grade (Fig. 8A). These results indicate that IL-6 expression in ductal epithelial cells is increased in more advanced stage of primary SS.

View larger version (44K): [in this window] [in a new window]   FIGURE 8. IL-6 expression and secretion by salivary gland epithelial cells. A, Characterization of IL-6 expression and histologic grading in LSG biopsy specimens from patients with primary SS. Immunohistochemistry for IL-6 was performed on 4-µm thick sections of grade 1 (left) and grade 4 (right) LSG biopsy specimens from patients with primary SS. Original magnification, x100. Inset magnification is x1000. A trend toward an increase of IL-6 expression in ductal epithelial cells (EP) with increasing histologic grading is shown. Grade 1 is characterized by slight infiltration and grade 4 displayed more than one focus per 4 mm3. Cellular aggregates with 50 or more lymphocytes, histiocytes, and plasma cells were defined as one focus. MN, mononuclear cells. B, Effect of S1P on IL-6 secretion from salivary gland epithelial cells. NS-SV-DC cells were treated with 0.01–0.5 µM S1P or with (+) IFN- (0.2 µg/ml) or left untreated (–). After 48 h of culture, culture supernatants were collected and IL-6 levels were measured by ELISA. Data represent mean ± SD from three independent experiments. *, p < 0.05.

Because SK1, S1P₁, and IL-6 are expressed in ductal epithelial cells from patients with primary SS (Figs. 2, 3, 8A), we examined the role of S1P₁ signaling for the secretion of IL-6 by ductal epithelial cells. IFN- significantly augmented IL-6 secretion by NS-SV-DC. Although low levels of S1P (0.01–0.1 µM) did not affect IL-6 secretion, higher levels of S1P (0.5 µM) significantly augmented IL-6 secretion by NS-SV-DC (Fig. 8B). These results indicate that IFN- and high concentrations of S1P induce IL-6 secretion by ductal epithelial cells.

Mediation of S1P-enhanced IFN- production by CD4⁺ T cells and Fas mRNA expression by NS-SV-DC cells via PTX-sensitive pathway

It has been reported that S1P₁ couple to PTX-sensitive G proteins of G_i/G₀ family (35, 36, 37). Because we demonstrated that both CD4⁺ T cells and salivary gland epithelial cells expressed S1P₁ (Figs. 2, 3, 4A), we investigated the role of PTX-sensitive G proteins in S1P enhancement of IFN- production by CD4⁺ T cells and Fas mRNA expression by NS-SV-DC cells. Peripheral blood CD4⁺ T cells were preincubated with 100 ng/ml PTX for 24 h. After rigorous washing, the cells were stimulated with plate-bound anti-CD3 mAb in the presence of S1P (0.01–0.5 µM). After 72 h, IFN- concentrations in culture supernatants were measured. Pretreatment with PTX inhibited S1P-enhanced IFN- secretion by CD4⁺ T cells (Fig. 9A). We next examined the effect of PTX-sensitive G proteins on S1P-enhanced Fas mRNA expression by NS-SV-DC cells. NS-SV-DC cells were preincubated with 100 ng/ml PTX for 24 h before S1P or IFN- stimulation. Pretreatment with PTX inhibited S1P enhancement of Fas mRNA expression by NS-SV-DC cells. However, preincubation with PTX did not affect the enhancing effect of IFN- on Fas mRNA expression by NS-SV-DC cells (Fig. 9B). These results indicate that S1P enhancements of IFN- production by CD4⁺ T cells and Fas mRNA expression by salivary gland epithelial cells depend on G_i/G₀-dependent pathway.

View larger version (19K): [in this window] [in a new window]   FIGURE 9. Effect of PTX on S1P-enhanced IFN- production by CD4+ T cells and Fas mRNA expression by salivary gland epithelial cells. A, IFN- production by CD4+ T cells with () or without () PTX pretreatment was measured using cells incubated with plate-bound anti-CD3 mAb (0.5 µg/ml) in the absence (–) or presence (+) of 0.01–0.5 µM S1P as described in Fig. 4C. After 48 h culture, culture supernatants were collected, and IFN- levels were measured by ELISA. Data represent mean ± SD from three independent experiments. *, p < 0.05. NS, Not significant. B, Fas mRNA expression by NS-SV-DC cells with () or without () PTX pretreatment was determined by treatment with S1P or IFN- for 6 h or left untreated as described in Fig. 7. Semiquantitative RT-PCR for the expression of Fas mRNA in NS-SV-DC cells was measured and were determined by normalizing expression with respect to GAPDH mRNA expression levels. Data represent mean ± SD from three independent experiments. *, p < 0.05. NS, Not significant.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

S1P concentrations in the lymph node and tissues (0.005–0.02 µM) are lower than those in lymph (0.03–0.3 µM) and in blood (0.1–1 µM). S1P concentrations in the lymph node and tissues are thought to enhance, whereas those in the blood suppress migration of T cells in murine model (14, 15). We observed that S1P (0.01–0.1 µM) enhanced proliferation and IFN- secretion by anti-CD3 mAb-stimulated CD4⁺ T cells, suggesting that concentrations of S1P in the tissues enhance IFN- production by TCR-stimulated CD4⁺ T cells. In contrast to our findings, Dorsam et al. (40) reported that proliferation and IFN- secretion by mouse CD4⁺ T cells stimulated with anti-CD3 mAb plus anti-CD28 mAb was inhibited by 0.001–1 µM S1P. This discrepancy may be explained by the different sensitivity of CD4⁺ T cell responses to S1P between mice and humans. Furthermore, we used a suboptimal dose of anti-CD3 mAb (0.5 µg/ml), whereas they used a much higher concentration of anti-CD3 mAb (2 µg/ml) for CD4⁺ T cell activation. Therefore, the enhancing effect of S1P on proliferation and IFN- secretion by CD4⁺ T cells may not be observed because of maximal CD4⁺ T cell activation by anti-CD3 mAb. Supporting our findings, Jin et al. (41) reported that S1P enhanced IL-2 and IFN- production by human peripheral blood T cells stimulated with anti-CD3 and anti-CD28 mAbs. We also observed that the enhancing effect of S1P on IFN- secretion by CD4⁺ T cells was stronger in patients with primary SS than in healthy controls. Taken together, increased S1P₁ signaling in infiltrating CD4⁺ T cells may enhance IFN- secretion by CD4⁺ T cells in the salivary glands of patients with primary SS.

Apoptosis of the acinar and ductal epithelial cells of the salivary and lacrimal glands has been proposed as a possible mechanism of primary SS. Apoptotic cell death may be induced by either CTLs through the release of proteases, such as perforin and granzyme B, or the interaction of Fas ligand expressed by T cells (42). Matsumura et al. (29) showed that IFN- and TNF- up-regulated Fas expression on human salivary gland epithelial cells. We also observed that IFN- up-regulated Fas mRNA expression in salivary gland epithelial cell line (NS-SV-DC). Interestingly, S1P (0.1–0.5 µM) up-regulated Fas mRNA expression in NS-SV-DC. Furthermore, S1P augmented IFN--induced Fas mRNA expression in NS-SV-DC. Caspase-3 appears to be indispensable for the apoptotic process (30). Both IFN- and S1P induced caspase-3 expression by NS-SV-DC in the presence of anti-Fas mAb. These results indicate that both IFN- and S1P augment Fas expression on salivary gland epithelial cells, thereby inducing apoptosis of the cells via Fas signaling.

The presence of various autoantibodies such as rheumatoid factor and anti-SSA/SSB Abs, as well as hypergammaglobulinemia, is considered to reflect B cell hyperactivity in primary SS. IL-6 is known to be a B cell growth and differentiation factor and it is generally found to be highly expressed in many autoimmune diseases (31). IL-6 mRNA is highly expressed in salivary gland of patients with primary SS (8). We observed IL-6 expression in ductal epithelial cells and inflammatory mononuclear cells. IL-6 expression in ductal epithelial cells was augmented in more advanced stages of primary SS. Furthermore, both IFN- and S1P augmented IL-6 secretion from a salivary gland epithelial cell line. These results suggest that S1P signaling augments IL-6 secretion from ductal epithelial cells in the salivary glands in patients with primary SS.

We investigated whether S1P-enhanced IFN- production by CD4⁺ T cells and Fas mRNA expression by salivary gland epithelial cells used S1P₁ signaling pathways. Both of these actions of S1P were inhibited by PTX. Because S1P₁ couples only to G_i, most of its effects are PTX sensitive, these results indicate that S1P₁ signaling pathways play an important role in modulating T cell as well as epithelial cell functions.

In conclusion, we have demonstrated increased S1P₁ expression in inflammatory mononuclear cells in the salivary glands of patients with primary SS. S1P₁ signaling enhanced proliferation and IFN- production by CD4⁺ T cells, Fas expression and Fas-mediated apoptosis by salivary gland epithelial cells, and IL-6 secretion by ductal epithelial cells. Therefore, S1P₁ signaling may play an important role in the pathogenesis of primary SS by potentiating IFN- secretion by CD4⁺ T cells, ductal epithelial cell apoptosis, and IL-6 secretion by ductal epitheliual cells. Regulation of S1P₁ signaling may be a novel therapeutic strategy in primary SS.

	Acknowledgment

 
We thank Sachie Kitano for technical assistance.

	Disclosures

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
The authors have no financial conflict of interest.

	Footnotes

 
The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

¹ This work was supported by Grant-in-Aid 17659306 for Exploratory Research from the Ministry of Education, Science and Culture of Japan.

² Address correspondence and reprint requests to Dr. Tsuyoshi Iwasaki, Division of Rheumatology and Clinical Immunology, Department of Internal Medicine, Hyogo College of Medicine, Mukogawa-cho, Nishinomiya, Hyogo 663-8501, Japan. E-mail address: tsuyo-i{at}hyo-med.ac.jp

³ Abbreviations used in this paper: SS, Sjögren’s syndrome; LSG, labial salivary gland; PTX, pertussis toxin; S1P, sphingosine 1-phosphate; SK, sphingosine kinase; GPCR, G protein-coupled receptor.

Received for publication November 14, 2007. Accepted for publication November 14, 2007.

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Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 

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