Pharmacologic doses of granulocyte colony-stimulating factor affect cytokine production by lymphocytes in vitro and in vivo

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Blood, Vol. 95 No. 7 (April 1), 2000: pp. 2269-2274
HEMATOPOIESIS

Pharmacologic doses of granulocyte colony-stimulating factor affect cytokine production by lymphocytes in vitro and in vivo

Elaine M. Sloand, Sonnie Kim, Jaroslaw P. Maciejewski, Fritz Van Rhee, Aniruddho Chaudhuri, John Barrett, and Neal S. Young
From the National Heart, Lung and Blood Institute, National Institutes of Health (NIH), Bethesda, MD.

  Abstract

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Peripheral blood stem cell (PBSC) transplantation is successful in improving engraftment without increasing acute graft-versus-hostdisease (GVHD), despite much larger numbers of T cells in unmanipulatedPBSCs than in bone marrow grafts. In mouse models and retrospectivehuman studies, granulocyte colony-stimulating factor (G-CSF) therapyhas been associated with less acute GVHD. We studied the effectof G-CSF on interferon (IFN)- $gamma$ and IL-4 expression in CD4⁺ lymphocytes. CD4⁺ cells co-cultivated with G-CSF and stimulated with PHA or CD3monoclonal antibodies showed significant decreases in IFN- $gamma$ andincreases in IL-4 expression (n = 13; P < .01). G-CSF appearedto have a direct effect on CD4⁺ cells independent of monocytes present in the culture becausepurified CD4⁺ cells exposed to G-CSF, washed, and cocultivated with untreatedmonocytes demonstrated similar changes in IFN- $gamma$ and IL-4 expression,whereas untreated CD4⁺ cells cocultured with G-CSF-stimulated monocytes behaved as controls.We then studied peripheral blood mononuclear cells (PBMCs) fromG-CSF-mobilized PBSC donors. When their PBMCs were cultured withPHA or CD3 monoclonal antibody, the percent of IFN- $gamma$ -expressingcells decreased by a mean of 55% and 42%, respectively, whereasthe percent of IL-4-containing cells increased by a mean of 39%and 58%, respectively, following G-CSF stimulation. Increasedapoptosis of IFN- $gamma$ -producing CD4⁺ cells was not responsible for the shift in TH1/TH2 subsets. G-CSF-RmRNA was present in both CD4⁺ and CD8⁺ cells. These results suggest that G-CSF decreases IFN- $gamma$ and increasesIL-4 production in vitro and in vivo and likely modulates a balancebetween TH1 and TH2 cells, an effect that may be important inPBSCtransplantation. (Blood. 2000;95:2269-2274)

© 2000 by The American Society of Hematology.

  Introduction

Top
Abstract
Introduction
Materials and methods
Results
Discussion
References

Use of peripheral blood stem cells (PBSC) for allogeneic bone marrow (BM) transplantation has a number of advantages overconventional BM grafting, including an improved yield of progenitorcells, ease of harvest, and shortened time to achieve engraftment.¹^,²Despite a 10-fold increase in the number of CD3⁺ cells in the apheresis product used for the transplantation ofstem cells, patients undergoing PBSC transplantation do not demonstratean apparent increased incidence or severity of acute graft-versus-hostdisease (GVHD).³^,⁴ This observation may be accounted forby a number of differences observed in BM and PB stem cells. PBSCobtained from granulocyte colony-stimulating factor (G-CSF)-mobilizeddonors contain more CD3⁺CD8CD4 cells than BM cells⁵; these cells decrease the severity ofacute GVHD in the murine model and are associated with decreasedcytotoxic lymphocyte activity in vitro.⁶ Similarly, monocytesobtained from G-CSF mobilized donors suppress cytotoxic responsesand T-cell proliferation when they are cocultivated with T cells.⁷^,⁸Recently, G-CSF was shown to polarize the balance within the murineT-lymphocyte subpopulations toward the TH2 cytokine productionin vitro.⁹

CD4⁺ lymphocytes can be functionally subdivided into TH1 and TH2 cells based on their pattern of cytokine expression.¹⁰ TH1cells can secrete tumor necrosis factor (TNF)- $alpha$ and IFN- $gamma$ , whereasTH2 cells are capable of producing IL-2, IL-4, and IL-10. Thebalance between these 2 subsets is altered in a number of pathophysiologicconditions and is associated with progression of or protectionagainst some infectious and autoimmune conditions.^11-13 Recentresults have suggested that acute GVHD is mediated by TH1 lymphocytesand that TH2 lymphocytes may exert a protective effect but mayhave a role in mediating chronic GHVD.¹⁴ In a murine model ofGVHD with TH1 and TH2 knock-out mice, TH1 cells mediated the symptomsof severe diarrhea and wasting, ultimately leading to death fromacute GVHD¹⁵; TH2 cells caused skin disease and were partiallyeffective in antagonizing the effect of TH1 cells. Experimentsusing the IFN- $gamma$ knockout mouse showed significant modificationof acute GVHD, confirming the importance of the role of IFN- $gamma$ .¹⁶

We hypothesized that G-CSF, in addition to its trophic effects on hematopoiesis, may have regulatory effects on T lymphocytesand may modulate immune responsiveness in unmanipulated PBSC graftsand autoimmune hematologic diseases in which it is used. Therefore,in this study we investigated the effects of G-CSF on TH1 andTH2 cell development in mitogen-stimulated human CD4⁺ cells and studied the mechanisms of G-CSF-mediated changes withinthe lymphocyte subpopulations. The in vitro findings were correlatedwith the effects of G-CSF on TH1 and TH2 lymphocyte distributionin PBSC donors receiving G-CSF for stem cellmobilization.

  Materials and methods

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Abstract
Introduction
Materials and methods
Results
Discussion
References

Stem cell donor selection and studies
Peripheral blood for in vitro studies was obtained from normal volunteers. For studies involving in vivo G-CSF stimulationof normal donors, samples were obtained from normal stem celldonors before and after 5 days of G-CSF treatment (10 µg/kg subcutaneouslydaily) before apheresis donation. Heparinized blood for cytokineexpression studies was obtained on day 1, before the administrationof G-CSF, and on day 6. In all cases, informed consent was obtainedaccording to protocols approved by the Institutional Review Boardof the National Heart, Lung, and Blood Institute. PBMC from G-CSF-stimulateddonors were separated as described below, and cells were culturedfor 48 hours with PHA (1 µg/mL) or anti-CD3 monoclonal antibody(mAb) (0.1 µg/mL). Cells were then surface stained with anti-CD4-phycoerythrin(PE) and intracellularly stained with either anti-IFN- $gamma$ -fluoresceinisothiocyanate (FITC) or anti-IL-4 FITC as describedbelow.

Cocultivation of G-CSF with T lymphocytes
Peripheral blood mononuclear cells (PBMCs) from normal unstimulated donors were separated using density gradient centrifugationwith lymphocyte separation media (Organon, Durham, NC). Cellswere washed twice with phosphate-buffered saline (PBS) and resuspendedin Iscove's modified medium supplemented with fetal calf serum(FCS; both Life Technologies, Gaithersburg, MD). Cultures of normalunstimulated donor cells were performed at a cell density of 0.5× 10⁶ cells/mL. When appropriate, natural lymphocyte-derived IL-2 (BoehringerMannheim, Indianapolis, IN) or phytohemagglutinin (PHA; BoehringerMannheim) were used for stimulation at concentrations of 20 U/mLor 8 µg/mL, respectively. G-CSF was used at a concentration of100 ng/mL (Amgen, Thousand Oaks, CA). GCSF was added to cultures;either PHA or CD3 mAb were added to cultures 24 hours later tostimulate cytokine expression. Cells were stained and enzyme-linkedimmunosorbent assay (ELISA) was performed on supernatants 2 dayslater.

Isolation of CD4⁺ cells, CD8⁺ cells, and monocytes. For lymphocyte subset separation, after washing with PBS supplemented with 2% human albumin, cells were applied to eithera CD4⁺ or a CD8⁺ affinity column (R&D Systems, Mineapolis, MN), and the cell fractionwas eluted with PBS according to manufacturer's instructions.An aliquot of eluted cells was stained with PE-conjugated anti-CD4or CD8 HPCA-12 mAb (Becton Dickinson, Mountain View, CA) to assesspurity. Monocytes were separated by adhesion to 250-mL polystyreneflasks in the presence of 20% FCS for 2 hours; this was followedby the removal of nonadherent cells and by PBS/2% FCS washes.Adherent cells were detached and resuspended by agitation at 4°Cin the presence of 1X Versene (BRL; Life Technologies). The usualpurity of the adhesion-separated monocytes ranged between 75%and 85% as determined by the expression of CD14⁺ antigens by flow cytometry. Cell viability was measured usinga standard trypan blue exclusion assay (LifeTechnologies).

Intracellular staining. Intracellular staining was performed on density gradient-separated PBMC. Intracellular staining for ICE expression was performedusing the Pharmingen Intracellular Staining Kit (Pharmingen).PBMC were stained with FITC-conjugated CD4 mAb and fixed. Aftermembrane permeabilization, cells were stained with PE-conjugatedanti-IFN- $gamma$ , anti-IL-4 mAb, or appropriate isotypic control mAb(Pharmingen). Permeabilization of cells was controlled using PermaSurereagents (Biosource). Samples were analyzed using an Epics ELITEflow cytometer(Coulter).

Apoptosis assay. Cultured PBMC were prepared as described above, washed with PBS, and stained with an annexin apoptosis kit (Pharmingen) accordingto the manufacturer's¹⁷ specifications and as previously described.Samples were analyzed using flowcytometry.

Cytokine ELISA
Concentrations of IL-4 and IFN- $gamma$ in tissue culture supernatants were measured using commercially available ELISA systems (R&DSystems). All determinations were made induplicate.

Reverse transcriptase-polymerase chain reaction for detection of G-CSF receptor expression
Peripheral blood mononuclear cells were sorted for CD4⁺ and CD8⁺ by flow cytometry. Total RNA was extracted using RNA STAT-60(Tel-Test, Friendswood, TX). Reverse transcription was performedusing an oligo d(T)₁₆ primer (RNA CORE KIT; Perkins-Elmer Cetus,Foster City, CA). After reverse transcription, the cDNA was amplifiedusing 5' and 3' primer pairs, 5'-AGTACAGTCCTCACCCTGATG-3', 5'-AAAGTATGCAGATCGCCTGGG-3'specific for G-CSF receptor.¹⁸ The following reverse transcriptionand amplification conditions were used: 42°C for 30 minutes, 99°Cfor 2 minutes, at 95°C for 1 minute, 55°C for 1 minute, and 72°Cfor 2 minutes for 40 cycles. PCR products were electrophoresedin 1% agarose gel, and the bands were visualized after stainingwith ethidium bromide and ultraviolet lightexposure.

  Results

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Abstract
Introduction
Materials and methods
Results
Discussion
References

G-CSF stimulated PBSC donors demonstrate decreases in IFN- $gamma$ and increases IL-4 expression in CD4⁺ cells
To determine whether G-CSF modulated the cytokine expression pattern of T lymphocytes, we used flow cytometry to examine intracellularcytokine expression in mononuclear cells derived from PBSC ofdonors receiving G-CSF. Normal donors receiving 10 µg/kg subcutaneouslydaily for 5 days were studied immediately before and after G-CSFadministration for PBSC donation by apheresis. After blood sampling,PBMCs were stimulated for 48 hours with either PHA or CD3 mAband were subsequently stained for intracellular IL-4 and IFN- $gamma$ .Donor CD4⁺ cells stimulated with G-CSF demonstrated significant changesin cytokine expression (Figures 1 and 2). In comparison to pretreatmentvalues, G-CSF increased IL-4 and decreased IFN- $gamma$ expression, resultingin a decreased TH1/TH2 ratio (determined by dividing the percentageof cells expressing IL-4 by the percentage of cells expressingIFN- $gamma$ ). In addition to a decreased proportion of cells expressingIFN- $gamma$ and an increased proportion of IL-4-expressing cells, therewere characteristic changes in the mean channel fluorescence (MCF)indicating changes in the intracellular cytokine content. IFN- $gamma$ and IL-4 MCF was measured on a relative scale (PHA-stimulatednormal lymphocytes showed MCF of 5 to 6, whereas isotype controlsregistered at less than 0.10). CD3 mAb-stimulated CD4⁺ cells from G-CSF-treated patients showed a mean decrease in MCFof $-$ 4.2 for IFN- $gamma$ , with a decrease in the percent of cells stainingby 42% with a concomitant increase in the number of cells stainingfor IL-4 by 58% with $Delta$ MCF = +6.0 (n = 10; P < .01). Determinationof IL-4 and IFN- $gamma$ concentrations in culture supernatants by ELISAresulted in similar changes (Table 1A).

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Fig 1. Effects of G-CSF administration on IFN- $gamma$ and IL-4 production by peripheral blood lymphocytes. Eleven normal stem cell donors received G-CSF (10 µg/kg per day) for 5 days. Blood was obtained before and after the administration of G-CSF. PBMC cells were purified by density-gradient centrifugation and were cultured with PHA for 48 hours. After permeabilization, cells were stained for IFN- $gamma$ and IL-4 as described in "Materials and methods." Scattergrams represent log PE (CD4 or CD8) fluorescence activity versus log FITC (IFN- $gamma$ and IL-4) fluorescence activity for representative donors (A, B).

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Fig 2. Effects of G-CSF on the percentages of CD4⁺ cells secreting IFN- $gamma$ and IL-4. Summary of the results obtained from 10 PBSC donors, including those exemplified in Figure 1. Bars represent percentages (mean ± SEM) in the IFN- $gamma$ and IL-4 expressing CD4⁺ cells before (black) and after (gray) treatment. Corresponding shifts in the mean fluorescence intensity for IFN- $gamma$ and IL-4 are described in the text. Statistical analysis (nonparametric Kruskal-Wallis test) for PHA: IL-4, P < .05; IFN- $gamma$ , P < .01. Statistical analysis for CD3 + IL-2: IL-4 P < .01; IFN- $gamma$ P < .01.


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Table 1. Production of IFN- $gamma$ and IL-4 in supernatants from cultures of peripheral blood mononuclear cells stimulated with G-CSF in vivo and in vitro

G-CSF decreased the proportion of IL-4 and IFN- $gamma$ producing lymphocytes in vitro
In a subsequent set of experiments, we asked whether the effects of G-CSF observed in PBSC donors could be replicated in vitro.Normal PBMCs were incubated with varying concentrations of G-CSF,then stimulated with IL-2 and CD3 mAb and stained 2 days laterwith CD4-PE and (after permeabilization) with either IL-4 or IFN- $gamma$ .Flow cytometric analysis showed that the number of CD4⁺ cells expressing IFN- $gamma$ decreased, whereas the number of IL-4-producingcells increased in cultures performed in the presence of G-CSF(Figure 3). The effect was less pronounced in cells that werenot preincubated with G-CSF before stimulation with either PHAor CD3 mAb (data not shown). The culture supernatants were alsotested for IFN- $gamma$ and IL-4 by ELISA. G-CSF resulted in changesin the cytokine production pattern that paralleled those detectedby flow cytometry (Table 1B). The effects of G-CSF were dosedependent (data not shown).

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Fig 3. In vitro effects of G-CSF on IFN- $gamma$ and IL-4 production. After exposure to G-CSF and polyclonal stimulation with PHA, IL-4 and IFN- $gamma$ expression were determined using flow cytometry as previously described. The columns represent the percentages (mean ± SEM) of cells expressing IFN- $gamma$ and IL-4. Summary of 13 experiments performed. Statistical analysis (nonparametric Kruskal-Wallis test) for IL-4: P < .01. Statistical analysis for IFN- $gamma$ : P < .01.

G-CSF has a direct effect on CD4⁺ cells
To determine whether the effects of G-CSF on cytokine production by T lymphocytes were directly mediated, we studied the growthfactor's effects on purified cell populations contained in PBMCpreparations. We compared IFN- $gamma$ expression in purified controlCD4⁺ and those treated by G-CSF after PHA stimulation. In the absenceof accessory cells, IFN- $gamma$ production was not detected in PHA-stimulatedCD4⁺ cells (data notshown).

When monocyte preparations, purified CD4⁺ cells, or CD8⁺ cells (98% pure by flow cytometry) were cultured in the presence ofG-CSF, washed, and then mixed $---$ G-CSF-exposed CD4⁺ cells with untreated monocytes; G-CSF-exposed monocytes withuntreated CD4⁺ cells not treated with G-CSF; G-CSF-exposed CD4⁺ cells with G-CSF-exposed monocytes $---$ and stimulated for 48 hourswith either CD3 mAb or PHA, only CD4⁺ cells directly exposed to G-CSF showed changes in IFN- $gamma$ expression(Figure 4 and Table 2). Neither CD4⁺ cells cultured with G-CSF-exposed monocytes nor CD8⁺ cells exposed directly or cultured with G-CSF-treated monocyteshad altered IFN- $gamma$ production.

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Fig 4. Direct effects of G-CSF on IFN- $gamma$ and IL-4 production by CD4⁺ T lymphocytes. Monocytes and CD4⁺ cells from normal donors were purified to obtain preparations with more than 98% purity as determined by flow cytometry using CD4 and CD14 mAb. Monocytes and CD4⁺ cells were separately exposed to G-CSF for 24 hours, washed, and mixed together (ratio 1:1). The expression of IFN- $gamma$ and IL-4 was measured using an intracellular staining technique and flow cytometry. Bars represent the changes (mean ± SEM) in the percentage of cells expressing IFN- $gamma$ (gray) and IL-4 (black) over a control mixture of monocytes and monocytes not exposed to G-CSF (summary of 2 independent experiments).


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Table 2. Direct effects of G-CSF on IFN- $gamma$ and IL-4 production by CD4⁺ T lymphocytes

G-CSF does not decrease TH1/TH2 ratio by increasing apoptosis
The G-CSF-induced modulation pattern of cytokine expression in CD4⁺ cells could potentially be mediated by the deletion of TH1 cellssecreting IFN- $gamma$ , as for example by selective apoptosis. Usingthe annexin technique, we investigated the effects of G-CSF onapoptosis of CD4⁺ cells. The presence of G-CSF in culture did not affect the numbersof apoptotic cells, as determined by flow cytometry. After 48hours of culture, a mean of 48% ± 10 TH1 cells and 54% ± TH2 cellsstained with annexin (n =3).

RT-PCR detects GCSF-R m-RNA expression in CD4 and CD8 cells
Peripheral blood mononuclear cells were sorted for CD4⁺ and CD8⁺ by FACS, resulting in a preparation that was 99.6% and 97% pure,respectively. Total RNA was extracted using RNA STAT-60, and RT-PCRwas performed using an oligo d(T)₁₆ primer. After reverse transcription,the cDNA was amplified using primer pairs 5'-AGTACAGTCCTCACCCTGATG-3'and 5'-AAAGTATGCAGATCGCCTGGG-3' specific for G-CSF receptor. Aband of 900 kbp was present for CD4 and CD8 cells, indicatingthe molecular presence of G-CSF-R (Figure 5).

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Fig 5. Expression of G-CSF mRNA in PB CD4⁺ and CD8⁺ cells. Purified CD4⁺ and CD8⁺ cells were derived by sorting PBMCs obtained from a normal healthy control. mRNA was extracted from the cells, and RT-PCR was performed using G-CSFR-specific primers. RT-PCR products were electrophoresed in agarose gel containing ethidium bromide and visualized under ultraviolet light. Unseparated normal bone marrow (nbm) from a normal control was used as a positive control.

  Discussion

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Abstract
Introduction
Materials and methods
Results
Discussion
References

In this study, we demonstrated that the pretreatment of T cells with G-CSF resulted in diminished IFN- $gamma$ and increased IL-4production when these cells were subsequently subjected to polyclonalstimulation with IL-2, PHA, or CD3 mAb in vitro. In the presenceof G-CSF, resting CD4⁺ cells that expressed low levels of IL-4 produced significantamounts of this cytokine after polyclonal activation. In agreementwith in vitro results, we found that when PBSC donors were stimulatedwith G-CSF for 5 days, their T cells produced less IFN- $gamma$ and moreIL-4 in comparison to pretreatment levels. This result impliesthat G-CSF decreased the TH1/TH2 ratio within the CD4⁺ T-cell population. Because monocytes constitute a major populationin PBSC harvests, they could in principle mediate the immunomodulatoryeffects of G-CSF on T lymphocytes. Using cocultivation experiments,we demonstrated that the effects of G-CSF on CD4⁺ T cells were direct and that monocytes were not required forG-CF-mediated modulation. Although previous results have shownthat monocytes undergo apoptosis as a result of exposure to IFN- $gamma$ ,survival of monocytes in our cultures was improved by their coculturewith G-CSF-treated CD4⁺ cells. This effect may have been caused by the diminished quantitiesof IFN- $gamma$ in G-CSF-supplemented cultures or the survival-promotingeffects of G-CSF. G-CF-mediated modulation of the cytokine patternproduced by T cells could be related to apoptosis of a particularT-cell subset (either TH1 or TH2) or their preferential survival.From the lack of changes in the apoptosis rate of lymphocytesstimulated with G-CSF, we concluded that this cytokine exertsits effect on IFN- $gamma$ and IL-4 production through modulation ratherthan the preferential elimination of TH1cells.

Other investigators⁷^,⁸^,¹⁹ have demonstrated that G-CSF-mobilized monocytes exert inhibitory effects on T-cell proliferationand responsiveness. G-CSF-mobilized CD14⁺ cells express significantly lower levels of the costimulatatorymolecules B7-2, implying that low levels of B7-2 expression maycontribute to the decreasing T-cell responsiveness by providingsuboptimal amounts of stimulatory signals.⁸ The observationthat the blockade of B7 with soluble CD28 fusion protein leadsto subresponsiveness of the T cells also supports the theory thatG-CSF down-modulates the GVHD reactivity of PBSC grafts. Our resultsare not in contrast with this thesis, and both mechanisms maysimultaneously operate in PBSC donors, resulting in an unexpectedlow rate and intensity of GVHD in recipients of PBSC allografts.Another group²⁰ demonstrated the increased production of bothIL-4 and IFN- $gamma$ by PBMCs obtained from patients with non-Hodgkin'slymphoma who undergo autologous transplantation compared to normalcontrols. However, the contributions of the underlying disease,previous chemotherapy, and GCSF in changing cytokine responsivenesscannot be ascertained. In this study we showed that both CD4⁺ and CD8⁺ cells contain G-CSF receptor mRNA, suggesting a mechanism bywhich G-CSF directly interacts with Tcells.

Clinically, the use of unmanipulated PBSC transplants derived from donors treated with G-CSF is associated with an unexpectedlow rate of GVHD²^,³ given the relatively large number ofT cells infused. If G-CSF can mediate a shift in the balance betweenTH1 and TH2 cells, G-CSF administration to the PBSC donors mightinfluence the course of GVHD. Acute GVHD appears to be mediatedby TH1 cells and their proinflammatory cytokines IL-2, TNF, andIFN- $gamma$ .²¹ Although IFN- $gamma$ is a marker for TH1 cells, IFN- $gamma$ secretedby CD4⁺ and CD8⁺ donor T cells is one of the earliest events occurring in acuteGVHD.²² IFN- $gamma$ is thought responsible for the delayed hematopoieticrecovery and development of cytopenias.²²^,²³ IFN- $gamma$ is alsopresent in the intestinal lesions of acute GVHD, and anti-IFN- $gamma$ antibodies prevented bowel damage in a murine GVHD model. In contrast,TH2 cells appeared to favorably modify acute GVHD. IL-4, a productof TH2 cells, decreases the expression of other proinflammatorycytokines, which may lead to immunologic tolerance.²⁴ TH2 cells,however, may mediate chronicGVHD.

G-CSF also has been used to treat aplastic anemia. Especially in combination with SCF²⁵ or with antithymocyte globulin andcyclosporine,²⁶ G-CSF may have therapeutic activity apart fromits stimulatory effects on hematopoiesis. Both GVHD and aplasticanemia have been reported to be related to the overexpressionof IFN- $gamma$ .²⁷^,²⁸ For both, the beneficial effects of G-CSF maybe secondary to changes in IFN- $gamma$ production and the balance inthe TH1 and TH2 lymphocyte subsets. The effects of G-CSF on thecytokine secretion pattern of lymphocytes derived from G-CSF-treatednormal subjects were comparable to those observed in aplasticanemia. In studies to be reported elsewhere, we found that whenpatients with aplastic anemia and abnormally decreased TH1/TH2ratios were treated with G-CSF, significant changes in the TH1/TH2subsets were observed (unpublisheddata).

In summary, our results suggest that G-CSF, in addition to its stimulatory effects on hematopoiesis, can exert immunomodulatoryeffects on T lymphocytes, and these may be therapeutically exploitedin conditions associated with TH1/TH2 imbalance such as immune-mediatedbone marrow failure syndromes andGVHD.

  Footnotes

Submitted March 17, 1999; accepted December 2, 1999.

Reprints: Elaine M. Sloand, NIH, National Heart, Lung, and Blood Institute, 31 Center Dr, MSC 2490, Bldg 31, Room 4A11,Bethesda, MD 20892-2490; e-mail: sloande{at}nih.gov.

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

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Abstract
Introduction
Materials and methods
Results
Discussion
References

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