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Inhibition of Transmethylation Down-Regulates CD4 T Cell Activation and Curtails Development of Autoimmunity in a Model System

Brian R. Lawson^1,*, Yulia Manenkova^*, Jasimuddin Ahamed, Xiaoru Chen^*, Jian-Ping Zou, Roberto Baccala, Argyrios N. Theofilopoulos and Chong Yuan^*

^* Diazyme Laboratories Division, General Atomics, San Diego, CA 92186; Department of Immunology, The Scripps Research Institute, La Jolla, CA 92037; and Shanghai Institute of Materia Medica, Shanghai, China

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
Transmethylation affects several cellular events, including T cell activation, and blockade of this pathway may curtail inflammatory/autoimmune responses. Here, we demonstrate that transmethylation inhibition by a novel reversible S-adenosyl-L-homocysteine hydrolase inhibitor leads to immunosuppression by reducing phosphorylation of several key proteins involved in TCR signaling, including Akt, Erk1/2, and NF-B. Remarkably, this effect was largely restricted to CD4 T cells and correlated with reduced arginine methylation of Vav1, an essential guanine nucleotide exchange factor in T cell stimulation. Treatment with the transmethylation inhibitor averted, and even ameliorated, the CD4-mediated autoimmune disease, experimental autoimmune encephalomyelitis. The data suggest that transmethylation is required for CD4 T cell activation, and its inhibition may be a novel approach in the treatment of multiple sclerosis, and other CD4-mediated autoimmune diseases.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
Nucleic acid sequences rarely predict the final molecular state and activity of the encoded proteins, because posttranslational modifications frequently contribute essential functional characteristics (1). Although phosphorylation has long been studied as the major posttranslational modification, methylation, and in particular arginine methylation, has recently begun to attract attention and has been shown to affect many cellular processes by modifying not only proteins but also nucleic acids and phospholipids (2, 3, 4). The major transmethylation pathway involves methyltransferase-mediated donation of methyl groups by S-adenosylmethionine and conversion of S-adenosylmethionine to S-adenosyl-L-homocysteine (SAH),² a potent feed-back inhibitor of methyltransferases (5). This reaction is tightly regulated by S-adenosyl-L-homocysteine hydrolase (SAHase), a highly conserved ubiquitous enzyme that catalyzes the hydrolysis of SAH into adenosine and homocysteine.

Transmethylation is particularly important for the normal function of the immune system. For example, blockade of SAHase was associated with decreased Ig production and slower cell growth in a lymphoblastoid cell line (6) and decreased humoral and cell-mediated immune responses (7, 8, 9, 10). Mice deficient in the arginine methyltransferase CARM1 showed a partial developmental arrest in an early thymocyte progenitor subset (11). A critical role of transmethylation in the normal development and function of the immune system is further suggested by the human disease adenosine deaminase deficiency, in which the inability to convert adenosine to inosine is associated with an 50% reduction in SAHase activity (6). Lymphocytes appear to have a higher requirement for transmethylation reactions than other cell types, particularly when activated (12).

Initial findings of immunosuppression by transmethylation inhibition provided the impetus to identify clinically useful compounds to treat autoimmune/inflammatory diseases. A major hurdle in this effort was the irreversible action of such compounds and associated severe toxicity (5). Recently, however, we developed a potent, but reversible, SAHase-inhibiting compound (methyl 4-(adenin-9-yl)-2-hydroxybutanoate (DZ2002) and demonstrated its immunosuppressive activity (7, 8). This compound was rationally designed based on the x-ray crystal structure of SAHase (13), and computational binding studies which compared an irreversible SAHase inhibitor that reduced enzyme-bound NAD⁺ to NADH with a reversible SAHase inhibitor (D-Eritadenine) that did not reduce NAD⁺ to NADH or alter the structure of SAHase. DZ2002 was chosen from a panel of D-Eritadenine derivatives because of similar inhibitory activity (K_i 17 nM) (7), but with a larger k_off value (higher rate of dissociation) that renders it more reversible and less toxic.

The availability of this compound prompted us to further examine the mechanisms by which transmethylation inhibition induces immunosuppression and the potential therapeutic efficacy of this approach in a prototypic model of autoimmune disease, experimental autoimmune encephalomyelitis (EAE). This disease, primarily mediated by CD4 Th1 cells, can be induced in animals by the administration of myelin basic protein or other myelin protein derivatives, such as proteolipid protein (PLP_139–151) and myelin oligodendrocyte glycoprotein (MOG) and is considered a useful model for multiple sclerosis (14, 15, 16, 17, 18).

Here, we document that transmethylation inhibition interferes with both proximal and distal events in TCR signaling primarily in effector CD4 T cells, and we demonstrate the therapeutic efficacy of reversible transmethylation inhibition in EAE.

	Materials and Methods

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TCR signaling

Jurkat T cells (American Type Culture Collection), mouse total splenocytes, or isolated mouse CD4 and CD8 T cells were cultured overnight in serum-free medium to minimize background phosphorylations/methylations. Thereafter, cells were incubated with 100 µM DZ2002 or vehicle (0.4% DMSO in PBS) for 2 h and then stimulated with magnetic beads (Miltenyi Biotec) loaded with anti-CD2, -CD3, and -CD28 (all Abs at 100 µg/ml) for intervals up to 1 h. In preliminary experiments, treatment with DZ2002 at concentrations up to 1 mM did not cause either apoptosis or necrosis in primary cultured T cells or cell lines for up to 24 h (data not shown). Protein was extracted in the presence of protease and phosphatase inhibitors (Pierce Biotechnology), and quantitated by the Bradford assay (Bio-Rad). Proteins were then separated on 4–12% SDS-PAGE polyacrylamide gels (20 µg/lane), transferred onto polyvinylidene difluoride membranes, blocked with nonfat milk powder, and probed with Abs to total and then phosphorylated Akt, Erk1/2, NF-B, Lck, STAT1, and STAT3 (all from Cell Signaling Technology). After membranes were initially probed with Abs to total protein levels, most membranes were stripped and reprobed for anti-phosphorylated protein levels, although in a few instances separate gels were run. Bands were revealed with secondary anti-rabbit or anti-mouse IgG-HRP Abs (BioLegend) as appropriate and developed for chemiluminescence. Membranes were then stripped and probed with anti--actin Abs (BioLegend) to confirm equal protein loading.

For Vav1 methylation assessment, cleared protein lysates were immunoprecipitated with anti-mono and dimethyl arginine (DMA) Abs (Abcam), and methylated proteins were isolated with protein G. Washed beads were separated on an 8–16% SDS-PAGE gel and immunoblotted with anti-Vav1 Ab (Santa Cruz Biosciences; Ref. 19). Proteins were visualized by Super Signal West-Femto Chemiluminescent Substrate (Pierce Biotechnology), and digitized using an Epson Perfection 48700 PHOTO scanner. To control for gel loading, cleared lysates were analyzed for -actin (Fig. 2) as well as total Vav1 protein levels, which were equal (data not shown).

View larger version (38K): [in this window] [in a new window]   FIGURE 2. DZ2002 inhibits Vav1 methylation in CD4 T cells. A, Mouse CD4 T cells or human Jurkat cells were pretreated with DZ2002 for 2 h and then activated with beads loaded with anti-CD2, -CD3, and -CD28 for 60 min. Protein lysates were immunoprecipitated (IP) with anti-DMA (-DMA) or anti-Vav1 Abs as indicated and immunoblotted for Vav1 or DMA, correspondingly. Actin from the original protein lysates was used to control for protein loading. B, Quantitation of bands (mean ± SEM) from A at 30 min. *, p < 0.05. Data are representative of three independent experiments.

Mouse splenocytes were pretreated with either 100 µM DZ2002 or vehicle for 2 h at 37°C. Cells were then loaded with Indo-1, acetoxymethyl ester (2 µg/ml) dissolved in pluronic-127 in the presence of probenecid (4 mM), all from Invitrogen, for 30 min at room temperature in the dark and labeled with CD4-PE, CD8-allophycocyanin, and biotinylated anti-CD3 and -CD28 (all from BioLegend). Each sample was warmed to 37°C before analysis. Baseline fluorescence was monitored for 2 min before addition of avidin (60 µg/ml; Vector Laboratories) to cross-link the biotinylated anti-CD3/CD28 Abs (20). Calcium flux data were acquired for 10–15 min at 351 nm on a LSR II flow cytometer (BD Biosciences) and analyzed with FlowJo software.

Short hairpin RNA (shRNA) transfections/RT-PCR

Jurkat T cells were transfected using Lipofectamine 2000 (Invitrogen) with plasmids containing the neo gene and shRNAs targeting the gene encoding SAHase (Ahcy; Superarray Biosciences), and stable transfectants were selected with G418. Knockdown of Ahcy was confirmed by quantitative RT-PCR (21). Briefly, RNA was isolated from several control and Ahcy knockdown transfectants, cDNA synthesis was performed, primers to Ahcy, a housekeeping gene, and a nonsense control sequence were mixed with SYBR Green, and samples were analyzed on a Rotor Gene 3000 (Corbett Research) after 45 cycles. Selected transfectants and nontransfected Jurkat cells were then stimulated with plate-bound anti-CD3 (5 µg/ml) and PMA (50 ng/ml), and CD69 expression (very early activation Ag) and IL-2 levels were analyzed by FACS (16 h later) or by ELISA (48 h later), respectively.

DZ2002 washout experiment

Jurkat T cells were pretreated or not with DZ2002 (100 µM) for 2 h after which DZ2002 was removed by washing in fresh growth medium three times. Cells were allowed to rest for an additional 2 h; then cells were stimulated with anti-CD2-, -CD3-, and -CD28-coated beads (Miltenyi Biotec), and protein lysates were analyzed for phosphorylated Akt (Cell Signaling Technology) 10 min after activation as described above. Phosphorylated Akt levels in the vehicle-treated cells were set as 100% expression and DZ2002 and DZ2002 wash-out levels are depicted as a percentage of control values.

In vitro SAHase inhibition assay

The SAHase inhibitor or its inactive analog was dissolved in vehicle. The assay reaction contained 50 mM phosphate buffer (pH 7.4), 320 µM SAH, 100 µM 5',5'-dithiobis(2-nitrobenzoic acid), 50 µg SAHase, and 0.5 µM DZ2002, 0.5 µM analog, or vehicle. Optical density was recorded at 405 nm at room temperature from 0 to 7 min on a UV-1601PC spectrophotometer (Shimadzu; Ref. 7). K_i was calculated by the equation K_i = K_obs/ (1 + [substrate]/K_m) in which K_obs = [inhibitor]/(V_o/V_i) – 1, and K_m = 7.9 µM.

Additionally, SAHase (0.5 mg/ml) was incubated with DZ2002 (100 µM) in 50 mM sodium phosphate buffer, pH 7.2, for 10 min at room temperature. SAHase and the SAHase-DZ2002 mixture were dialyzed against 50 mM sodium phosphate buffer, pH 7.2, for 24 h and the activity of SAHase was measured as above, both before and after dialysis.

Mice

Female SJL mice (4–6 wk old) were purchased from The Jackson Laboratory. Animals were housed in specific pathogen-free conditions, and all procedures were approved by The Torrey Pines Institute for Molecular Studies’ Animal Research Committee (La Jolla, CA).

EAE induction

Myelin PLP_139–151 (HSLGTKWLGHPDKF) was synthesized at NeoMPS, and 4 mg/ml of this peptide in PBS were emulsified 1:1 in IFA (Difco) supplemented with 4 mg/ml Mycobacterium tuberculosis (HRA-37; Difco); 100 µl of emulsion containing 200 µg of PLP_139–151 were injected s.c. into three different spots on the backs of female SJL mice (10 mice/group). Additionally, 200 ng of pertussis toxin (PTX) in PBS were administered i.p. on days 0 and 2 (22). Mice were monitored daily, and paralysis was scored blindly according to the following criteria: 0, no observable disease; 1, limp tail; 2, limp tail and partial weakness; 3, one hind limb paralyzed; 4, both hind limbs paralyzed; and 5, moribund or dead (23).

Adoptive transfer of EAE

Donor female SJL mice (n = 10) were immunized with 200 µg of PLP_139–151 in CFA as above, and reimmunized on day 7 with PLP_139–151 in IFA (Difco). Spleens were harvested on day 10, RBCs were lysed, and cells (5 x 10⁶ cells/ml) were cultured in RPMI-10% FBS, supplemented with 30 µg/ml PLP_139–151, and 10 ng/ml recombinant mouse IL-12 (BioLegend). After 96 h, cells were washed, resuspended in PBS, and injected i.p. (7.2 x 10⁶ cells/mouse) into 6- to 8-wk-old female SJL naive recipient mice (n = 10 mice/treatment group; Ref. 22). PTX was administered to these recipients on days 0 and 2, and disease severity was scored as indicated above.

Treatment protocols

The SAHase inhibitor DZ2002 was synthesized at Diazyme Laboratories, dissolved in vehicle, and delivered either i.p. (50 mg/kg/day) or s.c. by implanted osmotic pump (Alzet) at 0, 0.1, 1, and 10 mg/kg/day. Osmotic pump DZ2002 concentration was calculated on the basis of osmotic pump daily release rate and total mouse body weight. Prophylactic treatment (osmotic pump delivery of DZ2002) was initiated simultaneously with the initial PLP_139–151 immunization, whereas therapeutic treatment (i.p. delivery of DZ2002) began only after clinical symptoms began to appear (day 11 post-PLP_139–151 challenge; disease score, 1). The dosage of DZ2002 was determined by a preliminary acute toxicity study, which indicated that the LD₅₀ of DZ2002 administered i.p. was 520 mg/kg/day (data not shown). We administered 10 times less than the LD₅₀ and, indeed, observed no signs of overt toxicity in any mice over the course of these studies. Additionally, mice treated for 9 mo with daily i.p. injections of DZ2002 (50 mg/kg/day) also showed no signs of toxicity (data not shown).

To confirm that the mechanism of immunosuppression was inhibition of SAHase, a DZ2002 analog lacking the SAHase-inhibitory activity of DZ2002 was also synthesized, and administered at 10 mg/kg/day by osmotic pump.

Histology

DZ2002- and vehicle-treated mice were sacrificed on day 13 (the peak of disease in the control group) and perfused with PBS, and spinal cords were extracted and fixed in 10% buffered formalin. Paraffin-embedded, 4-µm-thick sections of mouse spinal cord were Luxol-fast blue stained to determine immune cell infiltration and degree of demyelination. Complete histological examination was also performed.

FACS

Splenocytes were harvested on day 13 post-PLP_139–151 challenge, and RBCs were lysed in ammonium chloride solution and stained with Abs to CD4, CD8, CD19, CD25, CD29 (VLA-4 -chain), CD40, CD40L, CD44, CD49d (VLA-4 -chain), CD69, CD80, CD86 (all from BioLegend), or F4/80 (Caltag). For intracellular cytokine analysis, splenocytes were stimulated with PLP (10 µg/ml) for 48 h, treated with brefeldin A (3 µg/ml), and stained with Abs to CD4, CD8, or CD19. After fixation and permeabilization, cells were stained with allophycocyanin-conjugated Abs to IL-2, IL-4, IL-10, IFN-. or TNF- (all from BioLegend). Cells were acquired on a FACSCalibur (BD Biosciences) and analyzed using CellQuest software (BD Biosciences).

Acute and recall responses to PLP_139–151

For acute EAE responses, disease was induced, and mice were treated with either DZ2002 or vehicle for 13 days (10 mice/treatment group). For recall EAE responses, disease was induced, and mice were treated with either DZ2002 or vehicle for 42 days (10 mice/treatment group). At the indicated times, spleens were harvested, and cells were stimulated in vitro on microtiter plates (2 x 10⁵ cells/well) with PLP_139–151 (10 µg/ml) for 72 h at which time WST-8 reagent was added according to the manufacturer’s instructions (Dojindo). OD was read at 450 nm. WST-8 is bioreduced by cellular dehydrogenases to an orange formazan product. The amount of formazan produced is directly proportional to the number of living cells, and the detection sensitivity of cell proliferation using WST-8 was shown to be equivalent to the thymidine incorporation assay.

Similar cultures were set, and supernatants were collected at 48 h and assessed by ELISA for the presence of IL-2, IL-4, IL-10, IFN-, and TNF- using commercially available Ab pairs (BioLegend).

Statistics

EAE disease severity scores are depicted as the average of the treatment group per day over the treatment period and were analyzed using the Kruskal-Wallis test. All other group mean comparisons were conducted using Student’s t test. Statistical analyses were performed using MedCalc for Windows, version 8.1.0.0 (MedCalc Software). p < 0.05 was considered significant.

	Results

Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 
Inhibition of SAHase reduces TCR signaling

Immunosuppression mediated by transmethylation inhibition may be due to interference with proximal and/or distal events associated with TCR signaling. To examine this possibility, we cultured total splenocytes from SJL mice in the presence or absence of the reversible SAHase inhibitor, DZ2002 for 2 h and then stimulated these cells with anti-CD2-, -CD3-, and -CD28-coated beads. Protein lysates were prepared at intervals for up to 1 h and assessed for levels of relevant phosphoproteins. We observed significant reductions in phosphorylated Akt and Erk1/2, whereas phosphorylated NF-B, Lck, STAT1, and STAT3 were unaffected (Fig. 1, A and B).

View larger version (53K): [in this window] [in a new window]   FIGURE 1. Inhibition of SAHase impairs TCR signaling. A, Phosphorylation (P) of TCR signaling proteins from mouse splenocytes is depicted 10 min after activation with beads loaded with anti-CD2, -CD3, and -CD28. B, Quantitation of bands (mean ± SEM) from A. *, p < 0.05. C, Phosphorylation (P) of TCR signaling proteins in mouse CD4 or CD8 T cells is depicted 10 min after activation with beads loaded with anti-CD2, -CD3, and -CD28. D, Quantitation of bands (mean ± SEM) from C. *, p < 0.05. E, Calcium mobilization in mouse CD4 and CD8 T cells pretreated with either vehicle or DZ2002 and activated with anti-CD3 and -CD28. Data are representative of three independent experiments.

To evaluate whether decreases in TCR signaling by transmethylation inhibition were T cell lineage specific, we repeated the above experiments with purified (>95%) CD4 and CD8 T cells. Strikingly, substantial reductions in phosphorylated Akt (16.1-fold), Erk1/2 (8.4-fold), and NF-B (2.1-fold) were restricted to the DZ2002-treated CD4 subset, whereas the DZ2002-treated CD8 T cells showed increases in these phosphoproteins (Fig. 1, C and D).

Inhibition of transmethylation reduces calcium mobilization by activated CD4 T cells

Reductions in TCR signaling induced by transmethylation inhibition will likely be reflected by the intensity of calcium mobilization. To assess calcium flux, primary T cells were pretreated for 2 h with either vehicle or DZ2002 and activated with anti-CD3 and -CD28, and the intensity of calcium mobilization was measured. Calcium mobilization was significantly reduced in DZ2002-treated CD4 T cells with the area under the induction curve being 44.5% less than the control cells (Fig. 1E). Contrastingly, the reduction in calcium flux of DZ2002-treated CD8 T cells was more modest (16.2%).

Vav1 methylation is SAHase dependent

It has been demonstrated that CD28 engagement induces protein arginine methyltransferase activity and the subsequent methylation of arginine on Vav1 (19). An irreversible inhibitor of SAHase reduced methylation of Vav1, resulting in decreased IL-2 production. Consistent with these findings, we found that a 2-h pretreatment with DZ2002 caused a decrease in Vav1 methylation of both naive mouse CD4 T cells and Jurkat cells. After activation with anti-CD3 and -CD28, this decline became even more evident at 30 and 60 min (Fig. 2A). Vav1 methylation of CD8 T cells appeared mostly unaffected by DZ2002 up to 30 min. Decreases in Vav1 methylation at 30 min were confined to the CD4 subset (Fig. 2B).

SAHase knockdown impairs T cell activation

To directly demonstrate that SAHase inhibition interferes with TCR signaling and T cell function, we transfected Jurkat T cells with shRNA targeting the gene encoding SAHase (Ahcy) or a nonsense control sequence. After activation, reductions in CD69 expression (Fig. 3A) and IL-2 production (Fig. 3B) were noted in the Ahcy knockdown transfectants (22% normal mRNA levels) compared with nonsense and nontransfected Jurkat T cells. Smaller reductions in CD69 expression and IL-2 production were also noted in DZ2002-treated Jurkat cells (data not shown).

View larger version (18K): [in this window] [in a new window]   FIGURE 3. Ahcy knockdown impairs T cell activation. A, Jurkat cells were transfected with shRNA targeting Ahcy mRNA or a nonsense control sequence and activated, and CD69 expression levels were determined (mean ± SEM). *, p < 0.05. B, Jurkat cells were transfected and activated as in A for 48 h, and supernatants were analyzed for IL-2 levels by ELISA (mean ± SEM). *, p < 0.05. Data are representative of three independent experiments.

DZ2002 is a reversible SAHase inhibitor

To document the reversibility of DZ2002, we cultured Jurkat T cells in the presence or absence of DZ2002 for 2 h, removed the compound and, after allowing cells to equilibrate for 2 more hours, stimulated these cells and assayed for levels of phosphorylated Akt. Once the SAHase inhibitor was removed, TCR signaling was restored in the DZ2002 washout cultures (Fig. 4A). As a confirmation of these results, we also incubated DZ2002 with SAHase, removed the compound by overnight dialysis, and showed that SAHase activity was almost fully recovered (Fig. 4B).

View larger version (18K): [in this window] [in a new window]   FIGURE 4. DZ2002 is a reversible SAHase inhibitor. A, Jurkat cells were cultured or not with DZ2002 for 2 h, washed to remove DZ2002, allowed to equilibrate for 2 additional hours, and then activated. Protein lysates were assayed for levels of phosphorylated Akt (mean ± SEM). *, p < 0.05. Untreated control Jurkat cells were used to set Akt levels at 100%. B, DZ2002 was first bound to SAHase (· · · · ·) or not (———) and enzyme activity was determined. The inhibitor/enzyme and control solutions were then dialyzed overnight with several buffer changes to remove DZ2002 after which enzyme activity was again determined (– · – · – ·). Data are representative of three independent experiments.

The results clearly indicate that the reversible transmethylation inhibitor DZ2002 potently suppresses T cell activation in a CD4-specific manner. Because EAE is mediated by myelin-recognizing CD4 T cells (14), we examined whether inhibition of transmethylation reactions could result in blockade and/or amelioration of this disease. EAE was induced by immunizing SJL/J mice with PLP_139–151 emulsified in CFA followed by PTX (22). A continuous supply of the inhibitor was ensured by s.c. implantation of osmotic pumps 3 days before EAE induction. Blockade of SAHase by DZ2002 (0.1–10 mg/kg/day) resulted in a significant dose-dependent reduction of EAE up to day 38, the last time of observation. Optimum effects were observed with doses of 10 (Fig. 5A) or 1 (Fig. 5B) mg/kg/day, but 0.1 mg/kg/day only had a modest effect (Fig. 5C). At day 14 (the peak of disease), DZ2002-treated mice showed an average disease severity score of 1.4 compared with 3.2 in the vehicle-treated controls. Moreover, the mean area under the disease severity curves showed an 2.3-fold overall reduction in the DZ2002-treated group, with 70% of the DZ2002-treated mice vs only 30% of the controls being disease-free by day 25 (Fig. 5D). Mice receiving the highest DZ2002 dose also showed an 3.1-fold decrease in infiltrating cells and a substantial reduction in demyelination compared with controls (Fig. 5E). The frequencies of total T or B cells in the spleens of treated animals were unaltered; however, there was a significant reduction in CD4, but not CD8, T cells expressing activation/memory markers (CD44^high and CD69) or integrin ₁ (Table I). Moreover, disease reduction by DZ2002 was due to SAHase inhibition because mice treated with an analog lacking a hydroxyl group and devoid of SAHase-inhibitory activity (Fig. 6A) was ineffective (Fig. 6B).

View larger version (58K): [in this window] [in a new window]   FIGURE 5. Reduction in SAHase activity protects mice from EAE. Group mean disease severity scores in vehicle (•)- and DZ2002 (A, 10 mg/kg/day) ()-, DZ2002 (B, 1 mg/kg/day; ()-, or DZ2002 (C, 0.1 mg/kg/day; )-treated mice; p < 0.0005 in A and B. In all panels, DZ2002 treatment began simultaneously (day 0) with EAE induction (10 mice/group). D, Percentage of mice in either group from A showing a score 1. E, Representative Luxol-fast blue- and H&E-stained fields of mouse spinal cords from control- and DZ2002-treated mice at day 14. Typical demyelination and mononuclear cell infiltrates are noted in control treated mice. Demyelination is indicated by loss of blue staining, whereas intact white matter is stained blue. Magnification, x400. Data are representative of four independent experiments.

View larger version (17K): [in this window] [in a new window]   FIGURE 6. DZ2002 is specific for SAHase. A, In vitro SAHase inhibition assay. Control (———), DZ2002 (· · · ·) or inactive analog (– – –). B, Group mean disease severity scores in vehicle (•)- and analog ()-treated mice (10 mice/group). Data are representative of two independent experiments.

Encouraged by the efficacy of DZ2002 in the treatment of acute EAE, we assessed whether this compound could also reduce established disease. EAE was induced, and at the first sign of disease (score, 1), mice were randomly assigned to either DZ2002- or vehicle-treated groups. In contrast to the preventive treatment protocol, DZ2002 (50 mg/kg/day) and vehicle were administered by i.p. injection once daily. This dose and injection schedule was based on previous observations that SAHase levels in liver were <50% of normal up to 24 h after administration of an SAHase inhibitor (5) and that such a regimen given for 9 mo had no discernable adverse effects (data not shown). By day 16 (peak of disease), both treatment groups showed similar severity scores (Fig. 7A). Strikingly, however, DZ2002-treated mice rapidly recovered, and by day 25 most of these mice were disease free with a mean score of 0.3 out to day 42. These data are in stark contrast to control animals that showed an overall incidence of 85% and a mean score of 1.5 at this time point (Fig. 7B). Moreover, comparison of the mean areas under the curves depicting disease severity showed an 2.4-fold reduction in DZ2002-treated mice compared with controls.

View larger version (22K): [in this window] [in a new window]   FIGURE 7. DZ2002 ameliorates both established and adoptively transferred EAE. A, Group mean disease severity scores in vehicle (•)- and DZ2002 ()-therapeutically treated mice (10 mice/group). DZ2002 was not administered until the animals began showing signs of disease (day 11; score, 1); p = 0.0024. B, Percentage of mice in either group from A showing a score of 1. C, Group mean disease severity scores in vehicle (•)- and DZ2002 ()-treated mice (10 mice/group) after transfer of encephalitogenic T cells; p < 0.0005. Data are representative of four independent experiments.

Inhibition of SAHase suppresses pathogenic T cells

EAE is transferable by encephalitogenic CD4 T cells (22). We used adoptive transfer experiments to determine whether SAHase blockade reduces the ability of pathogenic T cells to induce disease. Donor SJL mice were immunized with PLP_131–159 in CFA, and 10 days later splenocytes were restimulated in vitro with PLP_139–151 and IL-12. The resulting primed T cells (>95% CD3⁺) were injected (7 x 10⁶) into naive syngeneic recipients together with PTX on days 0 and 2. These mice were then treated or not with DZ2002 (50 mg/kg/day i.p.). Compared with controls, DZ2002-treated mice showed marked decreases in disease incidence (data not shown), onset, and severity, as indicated by an 2.6-fold reduction in the mean area under the curves depicting EAE scores (Fig. 7C). These results indicate that autoreactive T cells constitute a primary target for SAHase inhibition resulting in disease reduction.

SAHase inhibition suppresses proliferative and cytokine responses to PLP_139–151

To further document the effects of transmethylation inhibition on autoreactive T cells, we examined in vitro T cell proliferation and cytokine production in response to PLP_131–159 from splenocytes derived from mice at either the acute (day 13) or recall (day 42) phases of EAE. Compared with controls, DZ2002-treated mice at the acute phase showed a 70% reduction (Fig. 8A, left), and those at the recall phase a 50% reduction (Fig. 8B, left) in proliferative responses. Th1-type cytokines, thought to be involved in the pathogenesis of EAE (14), were also significantly reduced in DZ2002-treated cells at the acute phase, as indicated by both intracellular staining (Table I) and levels in supernatants (Fig. 8A, right). Thus, IL-2 (101.6 ± 17.6 vs 35.7 ± 3.8 pg/ml), IFN- (1,780.2 ± 78.4 vs 696.3 ± 40.9 pg/ml), TNF- (725.6 ± 89.4 vs 217.3 ± 16 pg/ml), and IL-12p40 (1,181 ± 235.2 vs 261.5 ± 68.2 pg/ml) were reduced, whereas IL-4 was somewhat increased (9.4 ± 2.1 vs >4 pg/ml). Because the IL-12p40 subunit is shared by IL-12 and IL-23, this reduction may be due to effects on either or both of these cytokines. Similar reductions in inflammatory cytokines, i.e., IL-2 (38.0 ± 3.7 vs 82.8 ± 8 pg/ml), IL-12p40 (94.6 ± 9 vs 192.8 ± 19 pg/ml), and TNF- (38.8 ± 3.5 vs 116 ± 11 pg/ml), albeit at lower levels, were also noted at the recall phase in the DZ2002-treated cells, but IL-4 and IFN- were undetectable in both treated and control cells at this phase (Fig. 8B, right).

View larger version (26K): [in this window] [in a new window]   FIGURE 8. Effect of transmethylation inhibition on ex vivo T cell proliferative and cytokine responses to PLP139–151. A, Splenocytes at the acute phase of EAE (day 14) were cultured with PLP139–151 (10 µg/ml). Cells were assayed for proliferative (left) and cytokine responses (right). B, Splenocytes at the recall phase of EAE (day 42) were cultured with PLP139–151 (10 µg/ml). Cells were assayed for proliferative (left) and cytokine responses (right). Data (10 mice/group) are given as mean ± SEM and represent two independent experiments; *, p < 0.05.

	Discussion

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Initially, the potential therapeutic utility of transmethylation inhibition focused on viral diseases (24, 25). More recently, however, applications to other clinical entities such as cardiovascular diseases, cancer, and autoimmunity have been considered (5, 7, 8, 26). Inhibition of transmethylation reactions may be accomplished either directly by blockade of methyltransferases, or indirectly by reducing SAHase activity. To date, however, designing specific methyltransferase inhibitors of clinical utility has been unsuccessful. Moreover, early classes of SAHase blockers acted irreversibly by either permanent trapping of the oxidized inhibitor onto the enzyme (type I), or by covalent modification of the active site of the enzyme (type II) (5). Although these compounds exhibited potent antiviral and immunosuppressive effects, the delay in reestablishing normal levels of SAHase (5 days; data not shown) led to severe toxicity, thereby precluding their clinical use. In fact, deletion of a segment on chromosome 2 in mice containing the Ahcy gene led to severe developmental defects that were reproduced in embryos cultured in the presence of an irreversible SAHase inhibitor or metabolites that elevate SAH (27). Therefore, efforts were made to develop reversible inhibitors of transmethylation, and among them DZ2002 was shown here, and previously, not to cause any overt toxicity, likely due to only 50% reductions in SAHase levels (8). In this regard, even in the case of more severe reductions in SAHase activity in humans due to genetic mutations, the associated metabolic defects were correctable by dietary restrictions and/or supplements (28).

Our in vitro studies showed that T cell signaling events were significantly reduced in DZ2002-treated T cells, including phosphorylation of Akt, Erk1/2, and NF-B and calcium mobilization. These effects appear to result from interference with Vav1 methylation, a guanine nucleotide exchange factor critical in the transduction of TCR signals (29). Others have also shown that Vav1 methylation accompanies CD28-costimulatory signaling and that this methylation allows nuclear translocation of Vav1 and subsequent increases in IL-2 production (19). In this report, however, superantigen-induced global tyrosine phosphorylation was shown to be unaltered by treatment with an irreversible SAHase inhibitor. The differences with our findings may primarily be attributed to the fact that Blanchet et al. assessed this parameter with total T cells, whereas we examined CD4 cells shown here to be the primary T cell target of transmethylation inhibition. Other, less likely possibilities include differences in the activation stimulus (superantigen vs anti-CD3/CD28) and the concentration of SAHase inhibitors (1 vs 100 µM).

Reductions in the proximal and distal events in TCR-signaling pathways were almost exclusively confined to the DZ2002-treated CD4 T cell subset. This finding supports the recent studies of Prisco et al. (30) in which mice carrying an arginine to glycine point mutation in the pleckstrin homology-domain of Vav1 showed selective CD4⁺, but not CD8⁺, perturbations in TCR-induced downstream activation pathways, despite the requirement of Vav1 in both lineages. No clear explanation for this lineage-specific effect of the pleckstrin homology domain mutation was provided, but the present findings suggest that differences in arginine methylation of this domain between CD4 and CD8 cells is the determining factor. In accordance with the above report, we suggest that Vav1 must be properly methylated before TCR activation; and in the absence of this posttranslational modification, TCR signaling through Vav1 is inhibited, at least in CD4 T cells.

The finding that transmethylation inhibition curtailed the effector function of CD4 T cells, and the previously noted higher methylation requirements in activated than resting T cells (9, 12), constituted the basis for assessing the effectiveness of DZ2002 in EAE, a model CD4-mediated autoimmune disease (14, 15, 16). DZ2002 was highly effective in reducing incidence, onset, and severity of not only acute but also established EAE, results highly compatible with our separate studies using MOG_35–55-immunized mice (31) and those of Moreno et al. (32), using a separate SAHase inhibitor, methylthioadenosine, in a rat model of EAE. In our MOG-induced model, we also observed a reduction in proliferation of DZ2002-treated T cells associated with the down-regulation of several cyclin-dependent kinases and up-regulation of a pancyclin inhibitor. The study using methylthioadenosine demonstrated reduced T cell proliferation, which was ascribed to a blockade in T cell signaling likely due to the prevention of IB- degradation and impaired activation of the NF-B pathway. Overall, these findings are in agreement with our current study, which further documents that SAHase inhibition causes deficits in TCR signaling by primarily affecting early signaling events dependent on Vav1 activation, particularly in the CD4 T cell subset.

These effects were clearly mediated by transmethylation inhibition, because a closely related analog devoid of SAHase-blocking activity was ineffective. These beneficial effects were associated with reductions in CNS infiltrates, demyelination, and acute and recall proliferative T cell responses to PLP_139–151. Th1-type cytokines (IL-2 and IFN-), thought to contribute to EAE pathogenesis, were also reduced. Others have previously reported that transmethylation inhibition interferes with gene transcription of several cytokines and attributed this to inefficient arginine methylation of STAT1 (33) and/or of the NF-AT cofactor protein, NIP45 (34). The disease-reducing effects of DZ2002 were unambiguously mediated by suppression of autoreactive T cells, because PLP_139–151-primed T cells were severely compromised in their ability to adoptively transfer EAE in DZ2002-treated recipients.

In addition to direct effects on activated T cells, inhibition of transmethylation may affect other processes in autoimmune/inflammatory responses. Indeed, we found a moderate impairment in chemokine-induced migration of DZ2002-treated monocytes (data not shown). This finding supports previous studies which showed that transmethylation reactions are required for effective recruitment of human monocytes to chemoattractants (35, 36). Thus, the beneficial effects of transmethylation inhibition may encompass reductions in the trafficking and homing of inflammatory cells into the CNS. Also, deimidation (the posttranslational conversion of positively charged arginine to neutral citrulline) and arginine methylation of myelin basic protein are increased in multiple sclerosis (1, 37), and it has been speculated that such posttranslational modifications of autoantigens in this and other autoimmune diseases, such as systemic lupus erythematosus (38), may provoke autoimmune responses. If so, transmethylation inhibition may reduce the availability of the inciting autoantigen(s).

In summary, we demonstrated that transmethylation inhibition suppresses CD4 T cell activation and that a reversible inhibitor of transmethylation effectively blocked EAE induction and, more clinically relevant, ameliorated established EAE. Considering that CD4 T cells are required in almost every autoimmune disease, reversible inhibition of transmethylation may have broad therapeutic potential, and indeed our current preliminary studies with DZ2002 indicate suppression of a lupus-like disease in a spontaneous mouse model.

	Acknowledgments

 
We thank Drs. Dennis R. Burton, Bruce Beutler, Laurie Owen, Nicholas R. J. Gascoigne, Kerri Mowen, and Dwight H. Kono for critical reading and review of the manuscript and Michael D. Wilson for statistical 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 Address correspondence and reprint requests to Dr. Brian R. Lawson at the current address: The Scripps Research Institute, Department of Immunology, IMM-3, 10550 North Torrey Pines Road, La Jolla CA 92037. E-mail address: blawson{at}scripps.edu

² Abbreviations used in this paper: SAH, S-adenosyl-L-homocysteine; SAHase, S-adenosyl-L-homocysteine hydrolase; DZ2002, methyl 4-(adenin-9-yl)-2-hydroxybutanoate; EAE, experimental autoimmune encephalomyelitis; PLP, proteolipid protein; MOG, myelin oligodendrocyte glycoprotein; shRNA, short hairpin RNA; PTX, pertussis toxin; DMA, mono and dimethyl arginine.

Received for publication November 27, 2006. Accepted for publication February 7, 2007.

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Top Abstract Introduction Materials and Methods Results Discussion Disclosures References

 

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