Differentiation of Tr1 cells by immature dendritic cells requires IL-10 but not CD25+CD4+ Tr cells

doi:10.1182/blood-2004-03-1211

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Blood, 1 February 2005, Vol. 105, No. 3, pp. 1162-1169.
Prepublished online as a Blood First Edition Paper on October 12, 2004; DOI 10.1182/blood-2004-03-1211.

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IMMUNOBIOLOGY
Differentiation of Tr1 cells by immature dendritic cells requires IL-10 but not CD25⁺CD4⁺ Tr cells
Megan K. Levings, Silvia Gregori, Eleonora Tresoldi, Sabrina Cazzaniga, Chiara Bonini, and Maria Grazia Roncarolo
From the San Raffaele Telethon Institute for Gene Therapy (HSR-TIGET); Cancer Immunotherapy and Gene Therapy Program, San Raffaele Scientific Institute; and Università Vita-Salute San Raffaele Milan, Italy.

   Abstract

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Dendritic cells (DCs) are specialized antigen-presenting cellsthat monitor the antigenic environment and activate naive Tcells. The role of DCs is not only to sense danger but alsoto tolerize the immune system to antigens encountered in theabsence of maturation/inflammatory stimuli. Indeed, if a naiveT cell encounters its antigen on immature DCs (iDCs), it maydifferentiate into a T-regulatory (Tr) rather than a T-effectorcell. However, little is known about the mechanisms by whichiDCs differentiate Tr cells. We developed a standardized andhighly reproducible protocol to differentiate Tr cells by repetitiveexposure of naive peripheral blood CD4⁺ T cells to allogeneiciDCs. The resultant Tr cells are phenotypically and functionallyidentical to type 1 Tr (Tr1) cells because their generationrequires production of IL-10 by iDCs, and they suppress T-cellresponses through an interleukin-10 (IL-10)– and a transforminggrowth factor ${beta}$ (TGF- ${beta}$ )–dependent mechanism. In addition,Tr1 cells induced by iDCs do not require the presence of CD4⁺CD25⁺Tr cells for their generation, nor do they express high constitutivelevels of CD25 or the transcription factor FoxP3. Thus, iDCscan drive the differentiation of Tr1 cells and can be used togenerate large numbers of alloantigen-specific Tr1 cells forclinical use as a cellular therapy to restore peripheral tolerance.

   Introduction

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Dendritic cells (DCs) are specialized antigen-presenting cells(APCs) that initiate immunity on encountering antigens associatedwith infection and inflammation.¹ This process requires theterminal maturation of DCs, typically induced by agents associatedwith microbial infection such as through the activation of Toll-likereceptor (TLR) and tumor necrosis factor receptor (TNF-R) familymembers. The resultant fully mature DCs are capable of primingnaive T cells to become effector T cells. More recently, thecapacity of DCs to influence T-cell differentiation in the absenceof inflammation has been explored. These studies have led tothe notion that immature or semimature DCs have a distinct rolein regulating immune responses because when they present antigens,they promote tolerance rather than immunity.^2,3
Peripheral T-cell tolerance can be induced and maintained bya variety of mechanisms, including deletion, induction of T-cellhyporesponsiveness, and differentiation of T-regulatory (Tr)cells. Tr cells include a wide variety of cells with a uniquecapacity to inhibit effector T-cell responses. Although T cellswith suppressive activity exist in essentially all T-cell subsets,CD4⁺ Tr cells are the best defined. Among these, CD4⁺CD25⁺ Trcells typically arise in the thymus, though some evidence indicatesthat they can also arise de novo in the periphery⁴ and can regulateT-cell responses through a cell contact–dependent mechanismyet to be defined.⁵ In contrast, CD4⁺ type 1 T-regulatory (Tr1)cells differentiate in the periphery from naive precursors,typically in the presence of interleukin-10 (IL-10), and ultimatelyregulate T-cell responses through their ability to produce IL-10and transforming growth factor- ${beta}$ (TGF- ${beta}$ ).^6,7 Several studies havereported that CD4⁺CD25⁺ Tr cells may also suppress responsesthrough the production of IL-10, TGF- ${beta}$ , or both,^8,9 leading tosome confusion regarding the relationship between CD4⁺CD25⁺Tr and Tr1 cells.⁵ However, recent data suggest that CD4⁺CD25⁺Tr and Tr1 cells are truly distinct subsets.¹⁰ Moreover, theobservation that CD4⁺CD25⁺ Tr cells may actually contributeto the differentiation of Tr1 cells in vitro^11,12 and in vivo¹³may call for reinterpretation of studies that found CD4⁺CD25⁺Tr cells mediated cytokine-dependent suppressive effects.
A great deal of interest has surrounded the hypothesis thatwhen DCs are in an immature or a "tolerogenic" state, they drivethe differentiation of these Tr cells. Indeed, targeting antigensto immature DCs in vivo through antibody-mediated delivery orinducible gene expression results in antigen-specific tolerancein CD4⁺ and CD8⁺ T cells.^14-18 This immature DC-induced toleranceappears to be caused by a combination of antigen-specific deletion^14,16,17and induction of Tr cells.^15,18 In addition, repetitive stimulationof cord blood CD4⁺ T cells with immature DCs results in thedifferentiation of Tr cells in vitro.¹⁹ Interestingly, thoughthe resultant Tr cells produce high levels of IL-10, their highlevels of expression of CD25 and CTLA-4 and their cell contact–dependentsuppression lead them to be classified as CD4⁺CD25⁺ Tr cellsrather than as Tr1 cells.
To define whether immature DCs induce the differentiation ofTr1 cells or CD4⁺CD25⁺ Tr cells, we investigated the effectsof repetitive priming of naive peripheral blood CD4⁺ T cellswith immature monocyte-derived DCs.

   Materials and methods

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Differentiation of DCs
Peripheral blood mononuclear cells (PBMCs) from healthy donorswere isolated by centrifugation over Ficoll-Hypaque gradients(Nycomed Amersham, Uppsala, Sweden). Approval was obtained fromthe San Raffaele Scientific Institute Institutional Review Boardfor these studies. In addition, informed consent was providedfor the use of blood samples according to the Declaration ofHelsinki. CD14⁺ monocytes were isolated as the adherent fractionafter incubation for 1 hour in RPMI 1640 (BioWhittaker, Verviers,Belgium) supplemented with 10% fetal calf serum (FCS) (BioWhittaker),100 U/mL penicillin/streptomycin (Bristol-Myers Squibb, Sermoneta,Italy), and 50 µM 2 mercaptoethanol (Bio-Rad, Segrate,Italy) (DC medium) at 37°C. After extensive washing, adherentmonocytes were differentiated into DCs by culture in 10 ng/mLrecombinant human IL-4 (rhIL-4) (R&D Systems, Minneapolis,MN) and 100 ng/mL recombinant human granulocyte macrophage–colony-stimulatingfactor (rhGM-CSF) (Schering-Plough, Kenilworth, NJ) in DC medium.After 5 days, DCs were left unstimulated or were transferredto wells containing irradiated (100 Gy) 3T3 fibroblasts expressinghuman CD40L (a kind gift from Vincenzo Russo) to induce maturation.After another 2 days, immature and mature DCs were collectedand irradiated at 60 Gy. DCs were either used directly or frozenuntil needed for restimulation. Purity and maturation stateof DCs were routinely checked by flow cytometric analysis todetermine the expression of CD1a, CD14, CD83, and HLA-DR. Typically,the cultures contained more than 90% CD1a⁺CD14^– cells.In some experiments, immature and mature DCs were also testedfor levels of expression of PD-L1, SLAM, and ILT-4 (kind giftsfrom Gregorio Aversa), ILT-3 (Immunotech, Marseilles, France),and CD45RB and CD45RO (BD Biosciences, San Jose, CA).
Purification of T cells
CD4⁺ T cells were purified from PBMCs by negative selectionusing the untouched CD4⁺ T cell isolation kit (Miltenyi Biotech,Auburn, CA), according to the manufacture's instructions. Aportion of the resultant CD4⁺ T cells was cryopreserved forlater use, and the remainder was depleted of CD45RO⁺ cells usinganti-CD45RO–coupled magnetic beads and LD negative-selectioncolumns (Miltenyi Biotech). Resultant cells were routinely morethan 90% CD4⁺CD45RO^–CD45RA⁺. For some experiments, theCD4⁺CD45RO^– T cells were subsequently depleted of CD25⁺cells using anti-CD25–coupled magnetic beads (MiltenyiBiotech).
T-cell differentiation
DCs (1 x 10⁵) were cultured with 1 x 10⁶ allogeneic CD4⁺CD45RO^–T cells in 1 mL X-vivo 15 medium (BioWhittaker), supplementedwith 5% pooled AB human serum (BioWhittaker) and 100 U/mL penicillin/streptomycin(Bristol-Myers Squibb). After 6 or 7 days, rhIL-2 (40 U/mL)(Chiron, Amsterdam, Holland) was added, and cells were expandedfor another 7 to 8 days. Fourteen days after initiation of theculture, T cells were collected, washed, and restimulated withimmature or mature DCs from the same allogeneic donor used inthe primary culture. After 3 days, rhIL-2 was added. One weekafter initiation of the second stimulation, T cells were collected,and a portion was tested for its proliferative and suppressivecapacity, whereas the remainder was restimulated a third time.In some experiments, neutralizing anti–IL-10R (3F9, 30µg/mL; BD PharMingen, San Diego, CA) monoclonal antibodies(mAbs) were added at the initiation of each round of stimulation,and each time the cells were split. T cells stimulated repeatedlywith immature DCs are referred to as T_(imm), and those stimulatedrepeatedly with mature DCs are referred to as T_(mat). Cultureswith immature DCs typically resulted in a 10-fold reductionin T-cell expansion compared with cultures stimulated with matureDCs. This reduced proliferation was not caused by increasedapoptosis (data not shown).
Transduction with lentiviral vector
Lentiviral vector was produced by calcium-phosphate transienttransfection of 293T cells using the pCCLsin.cPPT.hPGK ${Delta}$ NGFR.Wpreplasmid to confer expression of ${Delta}$ LNGFR as a cell surface markergene. CD4⁺CD45RO^– T cells were primed with immature ormature DCs, as described, and, after 5 days, the T cell/DC coculturewas transduced with lentiviral vector at a multiplicity of infectionof 20:1, in the presence of 8 µg/mL polybrene (Sigma,St Louis, MO) and IL-2 (40 U/mL). The next day, cells were collected,washed, and cultured for another 8 days. The percentage of transducedT cells was routinely approximately 20%. At the end of the 14-dayprimary stimulation period, the ${Delta}$ LNGFR⁺ T cells were purifiedby incubation with biotinylated anti–nerve growth factorreceptor (anti-NGFR) mAbs followed by streptavidin-coupled microbeadsand separation over magnetic columns (Miltenyi Biotech). Afterpurification, T cells, which were more than 90% ${Delta}$ LNGFR positive,were restimulated with immature DCs, as described.
Proliferation and suppression of T cells
To analyze the proliferative capacity of T_(imm) or T_(mat) inresponse to polyclonal activation, 96-well round-bottom plates(Costar, Cambridge, MA) were coated overnight at 4°C withanti-CD3 (OKT3; Jansen-Cilag, Raritan, NJ) mAbs (1 µg/mL)in 0.1 M Tris, pH 9.5, and were washed 3 times with phosphate-bufferedsaline (PBS). T cells were plated at an initial density of 2.5x 10⁵ cells/mL (50 000 cells/well) in a final volume of 200µL medium in the absence or presence of IL-2 (100 U/mL)and soluble anti-CD28 mAbs (1 µg/mL) (BD PharMingen).To test for the capacity of T_(imm) or T_(mat) cells to suppressproliferation or cytokine production, autologous CD4⁺ T cellswere thawed and stimulated with allogeneic mature DCs (10:1,T cells/DCs) or monocytes (CD3-depleted PBMCs, irradiated 60Gy) (1:1, T cells/monocytes). Naive CD4⁺ T cells were stimulatedalone or in the presence of T_(imm) or T_(mat) cells (1:1 ratio)in a final volume of 200 µL complete medium in 96-wellround-bottom plates. In some cultures, anti–IL-10R (30µg/mL, 3F9) or anti–TGF- ${beta}$ (50 µg/mL, 1D11;R&D Systems) mAbs, or both, were added. After the indicatedtime, either wells were pulsed for 16 hours with 1 µCi(0.037 MBq)/well [³H]-thymidine or supernatants were collectedfor analysis of interferon- ${gamma}$ (IFN- ${gamma}$ ) production.
To test for the suppressive capacity of T_(imm) cells by flowcytometry, naive CD4⁺ T cells were labeled with 5-(and-6)–carboxyfluorescein diacetate succinimidyl ester (CFSE) (Molecular Probes,Eugene, OR) and were stimulated with mature DCs at a 10:1 ratioin the presence of T_(imm) or T_(mat) cells. After 5 days, proliferationof the CFSE-labeled naive T cells was determined by flow cytometricanalysis. In some experiments, naive CD4⁺ T cells labeled withCFSE were stimulated with mature DCs at a 10:1 ratio in thepresence of absence of T_(imm) that had been transduced withlentivirus, as described. After 5 days, cocultures were stainedfor ${Delta}$ NGFR to distinguish the T_(imm) from the naive CD4⁺ T cells,and proliferation of the CFSE-labeled naive T cells was analyzedby flow cytometric.
ELISAs
T_(imm) and T_(mat) were stimulated with mature allogeneic DCsat a 10:1 ratio (T cells/DCs). Supernatants were collected after24 hours for IL-2 and IL-4, 48 hours for IL-10 and IFN- ${gamma}$ , and72 hours for TGF- ${beta}$ . To assess the amount of IL-10 produced byimmature DCs, DCs were cultured alone or with allogeneic CD4⁺T cells at a 10:1 ratio (T cells/DCs) in the presence or absenceof anti–IL-10R mAbs (30 µg/mL). Supernatants wereharvested after 48 hours. Levels of IL-2, IL-4, IL-10, and IFN- ${gamma}$ were determined by capture enzyme-linked immunosorbent assay(ELISA) according to the manufacturer's instructions (BD Biosciences).Levels of TGF- ${beta}$ in acidified supernatants were determined bycapture ELISA according to the manufacture's instructions (R&DSystems). The limits of detection were as follows: IL-2, 20pg/mL; IL-4, 20 pg/mL; IL-10, 20 pg/mL; IFN- ${gamma}$ , 60 pg/mL; andTGF- ${beta}$ , 60 pg/mL.
Quantitative PCR
Total RNA was extracted with Eurozol (Euroclone, Celbio, Milan,Italy), and cDNA was synthesized using the high-capacity cDNAarchive kit (Applied Biosystems, Foster City, CA). Levels ofFoxP3 and HPRT mRNA were quantitated using Assay on Demand real-timepolymerase chain reaction (PCR) kits (Applied Biosystems) withTaqMan Master Mix (Applied Biosystems). Samples were run induplicate, and relative expression of FoxP3 was determined bynormalizing to HPRT expression in each set of samples to calculatefold-change in value. mRNAs from freshly isolated CD4⁺CD25⁺Tr or CD4⁺CD25^– T cells were used as positive and negativecontrols, respectively.
Statistical analysis
All analyses for statistically significant differences wereperformed with the Student paired t test. P < .05 was consideredsignificant. All cultures were performed in triplicate, anderror bars represent the standard deviation.

   Results

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Cell surface phenotype of immature and mature DCs
We first performed extensive phenotypic analysis to confirmthe differentiation and maturation status of DCs. DCs were differentiatedfrom CD14⁺ monocytes in the presence of IL-4 and GM-CSF for5 days and were left unstimulated or were activated by coculturewith murine fibroblasts expressing CD40L for 48 hours. As expected,cultures of immature and mature DCs were routinely more than90% CD1a⁺CD14^– (Figure 1A). Immature DCs were CD83^–and HLA-DR^low; after activation for 48 hours by CD40 ligation,CD83 and HLA-DR were strongly up-regulated (Figure 1A). We nextdetermined whether molecules previously associated with tolerogenicDCs were expressed by immature or mature DCs. As previouslyreported, immature DCs expressed significantly lower levelsof PD-L1 compared with mature DCs (Figure 1B).²⁰ The mean fluorescenceintensity (MFI) of PD-L1 on immature DCs was 27.4 ± 11.6compared with 43.5 ± 10.9 for mature DCs (n = 4; P $≤$ .008).Similarly, immature DCs expressed low levels of SLAM, with MFIsof 9.6 ± 3.9 on immature DCs compared with 18.7 ±6.2 on mature DCs (n = 6; P $≤$ .02). In contrast, expression ofCD45RO, CD45RB, ILT-3, and ILT-4 was significantly higher onimmature DCs (Figure 1B). MFI of CD45RB on immature DCs was29.7 ± 15.5 compared with 13.7 ± 6.5 on matureDCs (n = 4; P $≤$ .03), expression of CD45RO was 17.2 ±5.7 on immature DCs compared with 9.3 ± 3.3 on matureDCs (n = 4; P $≤$ .01), expression of ILT-3 was 60 ± 22on immature DCs compared with 41 ± 20 on mature DCs (n= 4; P $≤$ .04), and expression of ILT-4 was 12.1 ± 4.0on immature DCs compared with 5.5 ± 3.9 on mature DCs(n = 5; P $≤$ .028).

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Figure 1.. Phenotype of immature and mature DCs. After 5 days of differentiation in IL-4 and GM-CSF, monocyte-derived DCs were left immature or were matured for 48 hours by the activation of CD40. DCs were then analyzed by flow cytometry to determine levels of expression of CD1a, CD14, CD83, and HLA-DR. (A) Percentages of positive cells, set according to the isotype-matched controls (not shown), are shown in each quadrant. (B) Expression of PD-L1, SLAM, CD45RO, CD45RB, ILT-4, and ILT-3 was also determined. Results are representative of (A) 17 and (B) 6 independent experiments.

Immature DCs induce T-cell hyporesponsiveness
We next standardized the protocol originally described by Jonuleitet al¹⁹ to determine the effects of repetitive stimulation ofperipheral blood CD4⁺CD45RO^– T cells with immature ormature DCs. CD4⁺CD45RO^– T cells were cocultured with DCsat a 10:1 ratio, as described in "Materials and methods," andsubsequently tested for their ability to proliferate in responseto mature DCs after 1, 2, or 3 rounds of stimulation. As shownin Figure 2A, with subsequent rounds of activation, T cellsprimed with allogeneic immature DCs became increasingly hyporesponsiveto reactivation with mature DCs. After 3 rounds of stimulation,an average reduction of 71% ± 5% (n = 17) in antigen-inducedproliferation was observed compared with T cells repetitivelyprimed with mature DCs. Similar results were obtained in responseto polyclonal activation (Figure 2B), with an average reductionin proliferation of 75% ± 5% (n = 17) after 3 roundsof activation with immature DCs. This hyporesponsiveness couldbe rescued by the addition of anti-CD28 mAbs and exogenous IL-2(Figure 2B).

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Figure 2.. Induction of T-cell hyporesponsiveness by immature DCs. Peripheral blood CD4⁺CD45RO^– T cells were stimulated with immature or mature allogeneic DCs 1, 2, or 3 times. (A) At the end of each stimulation period, T cells were tested for their ability to proliferate in response to mature allogeneic DCs. (B) In addition, after the third round of activation, their proliferative response to polyclonal activation was tested by stimulation with immobilized anti-CD3 mAb (1 µg/mL), in the absence or presence of soluble anti-CD28 mAb (1 µg/mL) and IL-2 (100 U/mL). After 48 hours of culture, [³H]-thymidine was added for an additional 16 hours. Results are representative of 17 independent experiments.

T_(imm) cells have suppressive capacity
The finding that repetitive in vitro stimulation of peripheralblood CD4⁺CD45RO^– T cells with immature DCs resulted inprofoundly hyporesponsive T cells suggested that these cellsmight also have acquired suppressive capacity. We thereforetested the ability of T_(imm) to suppress the responses of naiveautologous CD4⁺ T cells on challenge with allogeneic matureDCs. Naive CD4⁺ T cells were stimulated with mature DCs aloneor in the presence of T_(imm) or T_(mat) cells (1:1 ratio), andproliferation was assessed 1, 2, 3, or 4 days after initiationof the culture. Naive CD4⁺ T cells stimulated with mature DCsdisplayed the kinetics of a primary response, with proliferationpeaking after 4 days of culture (Figure 3A). As expected, T_(mat)cells generated in vitro using allogeneic mature DCs displayedthe kinetics of a secondary response when rechallenged withDCs from the same donor, with proliferation peaking at day 2.T_(imm) cells remained hyporesponsive throughout the time course.Adding T_(mat) cells to the primary mixed lymphocyte reaction(MLR) resulted in increased proliferation at day 2. Importantly,adding T_(imm) cells suppressed the proliferation of naive CD4⁺T cells in response to mature DCs. An average reduction of 69%± 19% (n = 13) in the proliferation of naive CD4⁺ T cellswas observed at 4 days after initiation of the culture. Thesedata were mirrored when we examined the production of IFN- ${gamma}$ :adding T_(mat) cells to the primary MLR resulted in an additiveeffect, whereas adding T_(imm) cells resulted in an almost completesuppression of IFN- ${gamma}$ production (Figure 3B).

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Figure 3.. Induction of Tr cells by immature DCs. Peripheral blood CD4⁺CD45RO^– T cells were stimulated 3 times with immature or mature allogeneic DCs. T cells were collected and tested for their ability to suppress responses of autologous CD4⁺ T cells. (A) Thawed CD4⁺ T cells were stimulated with mature DCs alone (MLR) or in the presence of T_(imm) or T_(mat) cell lines at a 1:1 ratio. [³H]-Thymidine was added at the indicated time for an additional 16 hours. (B) In parallel, supernatants were collected after 72 hours and analyzed by ELISA to determine levels of IFN- ${gamma}$ . (A-B) Results are representative of 17 independent experiments.

Because of the inability to independently assess the proliferationof T-cell lines and naive CD4⁺ T cells in thymidine assays,we also investigated the suppressive capacity of T_(imm) cellsusing CFSE-labeling and flow cytometric analysis. Adding T_(imm)cells to primary MLRs performed with CSFE-labeled naive CD4⁺T cells demonstrated that T_(imm) cells suppressed the proliferationof the naive cells, whereas adding T_(mat) cells resulted inan increase in the percentage of divided cells (Figure 4A).However, in these experiments, the inability to specificallygate on the naive CD4⁺ T cells made statistical analysis imprecise.We therefore performed similar experiments with T_(imm) cells,which were genetically marked with the truncated nerve growthfactor (NGF) R cell surface maker ( ${Delta}$ LNFGR) by lentiviral (LV)–mediatedgene transfer and thus could be excluded from the CSFE analysis.Five days after the initial stimulation with immature DCs, Tcells were transduced with LV- ${Delta}$ LNFGR. These experiments wereperformed with lentiviral vector rather than retroviral vectorto ensure that nondividing and dividing cells were transduced.9 days later, ${Delta}$ LNGFR⁺ T_(imm) cells were purified using magneticbeads, and cells were cultured and restimulated as described.At the end of the third round of activation, ${Delta}$ LNGFR⁺ T_(imm) cellswere tested for their ability to suppress proliferation of autologousCD4⁺ T cells, which were labeled with CFSE. As expected, adding ${Delta}$ LNGFR⁺ T_(imm) cells resulted in the profound suppression ofproliferation of the primary MLR (Figure 4B).

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Figure 4.. Suppressive activity of Tr cells by immature DCs. Naive CD4⁺ T cells labeled with CFSE were stimulated with mature DCs in the presence of T_(imm) or T_(mat) cells at a 1:1 ratio. (A) After 5 days of culture, the amount of proliferation was determined by flow cytometric analysis. (B) Naive CD4⁺ T cells were stimulated with immature DCs and infected with lentivirus encoding ${Delta}$ LNGFR 5 days after initiation of the culture. ${Delta}$ LNGFR⁺ cells were purified and restimulated with immature DCs twice. Autologous CD4⁺ T cells were labeled with CFSE and were stimulated with mature DCs in the absence or presence of a 1:1 ratio of ${Delta}$ LNGFR⁺ T_(imm) cells. After 5 days of coculture, the amount of proliferation of the naive CD4⁺ T cells was determined by flow cytometric analysis. Shown are histograms gated on NGFR-negative cells. Results are representative of 2 independent experiments.

Differentiation of Tr with immature DCs does not require naturally occurring CD4⁺CD25⁺ Tr cells
We tested whether there was a role for CD4⁺CD25⁺ Tr cells inthe induction of Tr cells from peripheral blood T cells. Thehighly purified CD4⁺CD45RO^– cells contained a small fraction(approximately 3%-5%) of CD25⁺ cells (Figure 5A). Thus we depletedCD25⁺ cells from CD4⁺CD45RO^– cells, and the 2 populationswere stimulated with immature DCs in parallel. Cultures initiatedwith both populations contained T cells that differentiatedinto Tr cells able to suppress the proliferation of naive autologousCD4⁺ T cells in response to mature DCs (Figure 5B). Furthermore,we could not detect a significant increase in expression ofCD25 on T_(imm) cells compared with control T_(mat) cells (datanot shown). To further exclude the possibility that T_(imm) cellswere similar to CD4⁺CD25⁺ Tr cells, we analyzed the levels ofexpression of the transcription factor FoxP3. In these experiments,levels of FoxP3 mRNA were expressed relative to those foundin highly purified CD4⁺CD25^– T cells and CD4⁺CD25⁺ Trcells, which provided a negative and a positive control, respectively.As shown in Figure 5C, FoxP3 mRNA is expressed at levels thatwere similar in T_(imm) and T_(mat) cells but that were significantlylower than those in freshly isolated CD4⁺CD25⁺ Tr cells. However,T_(imm) and T_(mat) cell lines did express more FoxP3 than freshlyisolated CD4⁺CD25^– Tr cells, a finding related to thefact that FoxP3 is up-regulated on activation in human T cells(Rosa Bacchetta, Laura Passerini, and M.G.R., unpublished data,May 2004). Together, these data indicate that peripheral bloodCD4⁺ Tr cells primed with immature DCs do not derive from, andare not equivalent to, CD4⁺CD25⁺ Tr cells.

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Figure 5.. CD25⁺ cells are dispensable for the differentiation of Tr cells by immature DCs. (A) Levels of CD25 expression on peripheral blood CD4⁺CD45RO^– or CD4⁺CD45RO^–CD25^– T cells were analyzed by flow cytometry. (B) Subsequently, CD4⁺CD45RO^– or CD4⁺CD45RO^–CD25^– T cells were stimulated with immature allogeneic DCs. At the end of 3 rounds of activation, T cells were collected and tested for their ability to suppress responses of autologous CD4⁺ T cells. Thawed CD4⁺ T cells were stimulated with mature DCs alone (MLR) or in the presence of a 1:1 ratio of T_(imm) or CD25^– T_(imm) cells. [³H]-Thymidine was added at the indicated time for an additional 16 hours. (C) T_(imm) cell lines were compared with T_(mat) cell lines for the expression of mRNA for FoxP3. Relative levels of FoxP3 expression were determined by quantitative real-time PCR. The amounts of FoxP3 mRNA are expressed as relative to CD4⁺CD25^– T cells (which were given an arbitrary value of 1). mRNA from freshly isolated CD4⁺CD25⁺ Tr cells was used as positive control. Results are representative of 3 independent experiments.

T_(imm) cells are phenotypically and functionally equivalent to Tr1 cells
Given that T cells primed by immature DCs did not appear tobe equivalent to CD4⁺CD25⁺ Tr cells, we next examined whetherthey had characteristics of IL-10–producing Tr1 cells.We first determined the cytokine production profile of T_(imm)and T_(mat) cells after activation with mature DCs. As shownin Table 1, T_(mat) cells produced all cytokines tested. In contrast,although T_(imm) cells clearly produced IL-10, IFN- ${gamma}$ , and TGF- ${beta}$ ,they consistently failed to produce significant levels of IL-2or IL-4. T_(imm) cells produced slightly lower amounts of IL-10compared with T_(mat) cells, whereas levels of TGF- ${beta}$ were notsignificantly different. Although T_(imm) cells did produce IFN- ${gamma}$ ,levels were at least 10-fold lower than those produced by T_(mat)cells. Thus, T_(imm) cells display a profile of cytokine productionsimilar to that of Tr1 cells: IL-10⁺IFN- ${gamma}$ ⁺TGF- ${beta}$ ⁺IL-2^–IL-4^–.

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Table 1.. Cytokine production profile of T_(imm) and T_(mat) cells

We next investigated whether the suppression of proliferationand cytokine production by T_(imm) cells was mediated throughthe production of IL-10, TGF- ${beta}$ , or both. We first performed suppressionexperiments as described in Figure 3A, in which naive CD4⁺ Tcells were activated with mature DCs in the absence or presenceof T_(imm) cells. Adding neutralizing anti–IL-10R and anti–TGF- ${beta}$ mAbs had little effect on the suppression of proliferation byT_(imm) cells (Figure 6A) but, importantly, completely reversedthe suppression of IFN- ${gamma}$ production on activation with matureDCs (Figure 6B). Adding isotype control antibodies had no effect(data not shown). Because it is well known that fully matureDCs are not susceptible to the inhibitory effects of IL-10 orTGF- ${beta}$ ,²¹ we subsequently performed parallel experiments usingallogeneic monocytes rather than mature DCs to induce the proliferationof naive T cells. Under these conditions, adding neutralizinganti–IL-10R and anti–TGF- ${beta}$ mAbs completely reversedthe suppression of proliferation (Figure 6C) and IFN- ${gamma}$ production(data not shown). Together, these data indicate that Tr cellsgenerated by repetitive stimulation with immature DCs are phenotypicallyand functionally equivalent to Tr1 cells.

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Figure 6.. Role of IL-10 and TGF- ${beta}$ in suppression mediated by T_(imm) cells. (A) After 3 rounds of activation with immature DCs, T_(imm) cells were tested for their ability to suppress the proliferation of CD4⁺ T cells in response to mature DCs, in the absence or presence of anti–IL-10R (30 µg/mL) and anti–TGF- ${beta}$ (50 µg/mL) mAbs. (B) Similar experiments were performed to assess the suppression of IFN- ${gamma}$ production by CD4⁺ T cells in response to mature DCs. (C) In parallel, proliferation and suppression in response to allogeneic monocytes was tested. [³H]-Thymidine was added at the indicated time for an additional 16 hours. Results are representative of 3 independent experiments.

Differentiation of Tr1 cells by immature DCs requires IL-10
IL-10 is a key differentiation factor for Tr1 cells.⁷ We investigatedwhether IL-10 was required for the generation of Tr1 cells inducedby immature DCs. CD4⁺CD45RO^– T cells were stimulated repetitivelywith immature DCs in the absence or presence of neutralizinganti–IL-10R or control immunoglobulin G (IgG) mAbs. Asshown in Figure 7A, the differentiation of T cells in the presenceof neutralizing anti–IL-10R mAbs completely reversed thehyporesponsive state, in terms of proliferation and IFN- ${gamma}$ production,induced by immature DCs. Moreover, the absence of IL-10 alsoprevented the induction of Tr cells with suppressive activity(Figure 7B).

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Figure 7.. Autocrine IL-10 is required for the differentiation of T_(imm) cells by immature DCs. Peripheral blood CD4⁺CD45RO^– T cells were stimulated with immature allogeneic DCs in the absence or presence of anti–IL-10R or control IgG mAbs (30 µg/mL). After 3 rounds of stimulation, T cells were collected and tested (A) for their ability to proliferate in response to mature DCs and (B) to suppress the response of autologous CD4⁺ T cells. [³H]-Thymidine was added after (A) 48 hours and (B) 72 hours for an additional 16 hours. In parallel, supernatants were collected after (A) 48 hours and (B) 72 hours, and IFN- ${gamma}$ secretion was measured by ELISA. Results are representative of 3 independent experiments.

Finally, we investigated the source of autocrine IL-10 in thesecultures. Although higher expression of IL-10 mRNA was detectedin immature DCs than in mature DCs (data not shown), we foundthat, as previously reported,²² significant levels of IL-10(Table 2) were produced by immature DCs, but only when blockinganti–IL-10R mAbs were added to the cultures. Adding Tcells to these cultures did not appreciably alter the amountof detectable IL-10 in the absence of presence of anti–IL-10RmAbs, indicating that most IL-10 is produced by immature DCs.

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Table 2.. Immature DCs produce autocrine IL-10

   Discussion

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Abstract
Introduction
Materials and methods
Results
Discussion
References

We analyzed the capacity of immature monocyte-derived DCs toinduce the differentiation of Tr cells from peripheral bloodCD4⁺ T cells. Together, our data strongly support the conclusionthat immature DCs drive the differentiation of IL-10–producingTr1, and not CD4⁺CD25⁺ Tr cells. Immature DCs produce autocrineIL-10, and, in conjunction with a unique combination of cellsurface molecules, this cytokine is essential for the differentiationof Tr1 cells. The resultant Tr1 cells produce IL-10, TGF- ${beta}$ , andIFN- ${gamma}$ , but they do not produce IL-4 or IL-2, nor do they expresshigh levels of FoxP3, and they are hyporesponsive to antigen-specificand polyclonal activation. This hyporesponsiveness can be reversedwith the addition of exogenous IL-2 and anti-CD28 mAb. Tr1 cellsinduced by immature DCs suppress proliferation and cytokineproduction by autologous CD4⁺ T cells through an IL-10–and a TGF- ${beta}$ –dependent mechanism. The presence of CD4⁺CD25⁺Tr cells was not required to differentiate Tr1 cells from immatureDCs, and the resultant Tr population did not express constitutivelevels of CD25 or FoxP3.
Our finding that repeated exposure to human immature DCs inducesthe differentiation of IL-10–producing Tr cells is similarto findings in previous reports.^18,19 However, in contrast toresults obtained with cord blood CD4⁺ T cells indicating thatwhen immature DCs were used to prime cord blood CD4⁺ T cells,the resultant Tr cells shared many characteristics with naturallyoccurring CD4⁺CD25⁺ Tr cells,¹⁹ we found that peripheral bloodT_(imm) cells mediated cytokine-dependent suppression and didnot acquire the phenotype of CD4⁺CD25⁺ Tr cells. The reasonfor this difference is unclear, but it is important to notethat the phenotypes of naive CD4⁺ T cells in peripheral andcord blood are distinct. Cord blood CD4⁺ T cells contain a significantlyhigher proportion of CD4⁺CD25⁺ Tr cells than peripheral bloodCD4⁺ T cells, and most are CD45RA⁺.²³ Furthermore, cord bloodT cells have an innate capacity to produce high levels of autocrineIL-10,²⁴ which we have previously shown can have a key rolein Tr1 cell differentiation.²⁵ Thus, it is possible that stimulatingcord blood CD4⁺ T cells with immature DCs might have resultedin a combination of expansion of preexisting CD4⁺CD25⁺ Tr cellsand differentiation of IL-10–producing Tr1 cells. In sucha mixed population, though IL-10 would have been detected, anyfunctional effects might have been masked by the presence ofcytokine-independent CD4⁺CD25⁺ Tr cells.
T_(imm) cells did not express constitutive CD25 or high levelsof mRNA for FoxP3, a transcription factor highly expressed inmouse and human CD4⁺CD25⁺ Tr cells.^26-28 Moreover, neither murinenor human IL-10–producing Tr cells express high levelsof FoxP3 mRNA^29,30 (see also Rosa Bacchetta, Laura Passerini,and M.G.R., unpublished data, May 2004). Thus, our data stronglysupport the conclusion that Tr cells induced by immature DCsare distinct from naturally occurring CD4⁺CD25⁺ Tr cells.
We have shown here that the effects of neutralizing anti–IL-10mAbs on the proliferation of CD4⁺ T cells should also be testedon stimulation with monocytes because mature DCs are not susceptibleto the suppressive effects of IL-10 produced by Tr1 cells.²¹Interestingly, though the blockade of IL-10 and TGF- ${beta}$ did notaffect the suppression of proliferation by T_(imm) cells, itcompletely restored the production of IFN- ${gamma}$ by CD4⁺ T cells activatedwith mature DCs. These data suggest that the mechanisms by whichTr1 cells suppress proliferation and cytokine production maybe distinct and that the suppression of cytokine productionmay be more prominent.³¹ Neutralizing anti–IL-10 and anti–TGF- ${beta}$ mAbs also reversed the anergic state of Tr1 cells (data notshown). These data are in accordance with previous findingsthat anti–IL-10 and anti–TGF- ${beta}$ mAbs can enhance theproliferative response of Tr1 cells.²⁵
Interestingly, the anergic state of Tr1 cells induced by immatureDCs was completely reversed on polyclonal activation in thepresence of anti-CD28 mAb and IL-2 but was maintained when thecells were activated with fully mature DCs. We can speculatethat the inability of fully mature DCs to revert the anergicstate of Tr1 cells induced by immature DCs is attributable toa lower strength of T-cell receptor (TCR) signaling than thatobtained with polyclonal stimulation using anti-CD3 and anti-CD28mAbs.
The mechanisms by which immature DCs promote the differentiationof Tr1 cells are not completely clear. As shown here, autocrineproduction of IL-10 is an essential component of the mechanism(Table 2; Figure 6). However, other molecules are clearly involvedbecause IL-10 alone is insufficient to induce the differentiationof Tr1 cells.²⁵ We found that, compared with mature DCs, immatureDCs express high levels of ILT-4 (Figure 1B), an inhibitorymolecule that binds to HLA-G and that is induced by IL-10³²and by ILT-3, which mediates the tolerogenic effects of DCsexposed to CD8⁺CD28^– T-suppressor cells.³³ Interestingly,CD45RB, a key marker for murine DCs that differentiate Tr1 cells,³⁴was also found to be significantly up-regulated on human immatureDCs, which induce Tr1 cells (Figure 1B). Conversely, immatureDCs expressed low levels of PD-L1 and SLAM (Figure 1B). Therefore,ILT-4 and ILT-3 or different isoforms of CD45 may play a rolein the induction of Tr1 cells by immature DCs.
Myeloid DCs can be made tolerogenic by a variety of means, includingtreating them with IL-10,³⁵ a combination of IL-10 and TGF- ${beta}$ ,³⁶or immunosuppressive agents such as vitamin D3³⁷; exposing themto certain types of bacteria³⁸ or certain endogenous proteinssuch as heavy chain ferritin³⁹; or transducing them with retroviralvectors that encode tolerogenic molecules such as IL-10, TGF- ${beta}$ ,CTLA-4, or Notch ligands.⁴⁰ In addition, specialized subsetsof DCs, which are strictly dedicated to tolerance induction,even in a mature state, can also induce Tr1 cells. For example,DEC205⁺B220⁺CD19^– DCs isolated from the liver and activatedin vitro with IL-3 and CD40 cross-linking induce Tr1 cells.⁴¹Similarly, human DC2 cells can induce the differentiation ofIL-10–producing CD8⁺ Tr cells.⁴² Whether the Tr cellsthat arise after stimulation with different types of tolerogenicDCs are phenotypically or functionally equivalent to the Tr1cells induced by immature DCs remains to be determined.
The requirement for multiple rounds of stimulation with immatureDCs to differentiate Tr1 cells is intriguing. The fact thatT cells must encounter tolerogenic DCs multiple times beforethey differentiate into Tr1 cells suggests that in vivo thismay be a safeguard to ensure that tolerance is only inducedtoward antigens consistently presented in a noninflammatoryenvironment.
In conclusion, immature DCs can efficiently differentiate andexpand antigen-specific Tr1 cells in vitro. These findings areconsistent with the idea that in the absence of inflammation,DCs function to tolerize the immune system to ingested/inhaledproteins and proteins derived from dying cells derived fromnormal cell turnover.⁴³ This level of control may also be operationalon CD8⁺ T cells.¹⁸ The fact that immature DCs induce IL-10–producingTr1 cells is consistent with the hypothesis that Tr1 cells areexclusively induced de novo in the periphery. The ability toexpand and genetically mark large numbers of alloantigen-specificTr1 cells is an important step toward the use of these cellsas therapy to induce tolerance after transplantation and inautoimmune diseases.

   Footnotes

Submitted April 1, 2004; accepted September 21, 2004.
Prepublished online as Blood First Edition Paper, October 12,2004; DOI 10.1182/blood-2004-03-1211.

Supported by a grant from the Italian Telethon Foundation.

M.K.L. and S.G. contributed equally to this study.

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 U.S.C. section 1734.

Reprints: Maria Grazia Roncarolo, HSR-TIGET, Via Olgettina 58, Milan, Italy 20132; e-mail: m.roncarolo{at}hsr.it.

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