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TRANSPLANTATION
From the Departments of Internal Medicine and
Pediatrics, University of Michigan Cancer Center, Ann Arbor; and the
Department of Pathology, Immunology, and Laboratory Medicine,
University of Florida, Gainesville.
Recent evidence suggests that dendritic cells (DCs) can regulate
and amplify immune responses. Flt3 ligand (FL)-derived DC function was
tested as a stimulator of allogeneic lymphocytes in vitro and in vivo.
Treatment of mice with FL dramatically expanded DC number, but DCs
isolated from FL-treated mice (FL DCs) were poor stimulators of
allogeneic T-cell responses in vitro. Further activation of FL DCs did
not restore their stimulatory ability, and FL DCs did not suppress the
stimulation of the allogeneic T cells by normal DCs. FL treatment
significantly increased the CD8 Flt3 ligand (FL) stimulates the proliferation of
hematopoietic progenitor cells through binding to the FL receptor,
which is restricted to cells of hematopoietic origin.1-3
Tissues in FL-treated mice display dramatic increases in DCs of
multiple organs, including spleen, lymph nodes, blood, thymus, liver,
lungs, Peyer patches, and bone marrow.4,5 Therefore, FL
has been proposed as a means to boost protective immunity against
several diseases including cancer and infectious agents. FL can augment immunologic responses,6-14 but it can also induce
tolerance.15
Dendritic cells (DCs) are centrally involved in the initiation of
T-cell-dependent immune responses. In mouse spleens, at least 2 major
subpopulations of DCs have been described, CD8 Given the controversy regarding FL effects on DCs and their control of
immune responses, we evaluated FL for its effects on DCs of allogeneic
T-cell responses as stimulators. We show that FL DCs, though increased
in number, only weakly stimulate allogeneic T-cell responses in vitro,
and this reduction is correlated with large increases in the
CD8 Mice
Flt3 ligand treatment
Isolation of DCs Spleens were injected with 0.5 mL collagenase D (1 mg/mL; Boehringer Mannheim, Indianapolis, IN) per spleen, cut into small pieces, and incubated for 45 minutes at 37°C. The resultant digested tissue suspension was teased through a 70-µm filter, centrifuged, and washed twice. In some experiments, cells were cultured overnight at 37°C and 5% CO2 in plastic tissue culture dishes to remove adherent macrophages. Next, the nonadherent cells were collected, resuspended in 1.035 g/mL Percoll (Pharmacia Biotech, Uppsala, Sweden), and underlain with an equivalent volume of 1.075 g/mL Percoll.20 After centrifugation, the resultant band was harvested and washed twice, and DCs were isolated by using CD11c (N418) MicroBeads and the autoMACS (Miltenyi Biotec, Bergisch Gladbach, Germany). In some experiments, these DCs were further separated according to their CD8 + expression, and 2 populations
(CD11c+ CD8+ and CD11c+
CD8 ) were sorted on a FACS Vantage SE cell sorter
(Becton Dickinson, San Jose, CA).
Flow cytometric analysis Monoclonal antibodies (mAbs) used were fluorescein isothiocyanate (FITC)-, phycoerythrin-, or allophycocyanin (APC)-conjugated anti-mouse CD45.1, CD3 , CD8, CD11b, CD11c
(HL3), CD25, CD40, CD49, CD80, CD86, and I-Ab (BD
PharMingen, San Diego, CA). Cells were preincubated with mAbs 2.4G2
(rat antimouse Fc R mAbs) for 15 minutes at 4°C to block
nonspecific FcR binding of labeled antibodies and then incubated
with the relevant mAbs for 30 minutes at 4°C. Finally, cells were
washed twice with 0.2% bovine serum albumin in phosphate-buffered saline, fixed with 1% paraformaldehyde in phosphate-buffered saline, and analyzed by EPICS Elite ESP cell sorter (Beckman-Coulter, Miami,
FL). Irrelevant IgG2a/b mAbs were used as a negative
control. Ten thousand live events were acquired for analysis.
Cell culture Splenic T cells were purified by passage through nylon wool columns (Polysciences, Warrington, PA) and then used as responders at 1 × 105 cells/well, together with graded numbers of irradiated (20 Gy) freshly isolated DCs. Percentages of CD11+ cells in the DC fraction were determined by flow cytometric analysis, and CD11c+ DC number was adjusted before placement in culture. Cultures were maintained in 10% heat-inactivated fetal calf serum in complete Dulbecco modified essential medium at 37°C in 7.5% CO2. After 1 to 5 days of culture, supernatants were harvested from the culture for cytokine measurement, and cells were pulsed with 3H-thymidine (1 µCi [0.037 MBq] per well) for an additional 16 hours. Proliferation was determined on a TopCount NTX (Packard Instrument, Meriden, CT).Enzyme-linked immunosorbent assay Enzyme-linked immunosorbent assay (ELISA) for interferon (IFN)-, IL-2, IL-4, IL-10, tumor necrosis factor- (BD
PharMingen), and IL-12 p70 (R&D Systems, Minneapolis, MN) were
performed according to the manufacturer's protocol. Briefly, samples
were diluted 1:1 to 1:4, and each cytokine was captured by the specific
primary mAbs and detected by biotinylated secondary mAbs. Assays were developed with avidin-horseradish peroxidase and substrate. Plates were read at 450 nm using a MAXLine microplate reader (Molecular Devices, Sunnyvale, CA). Samples and standards were run in duplicate, and the sensitivity of the assays was 31.3 pg/mL for IFN-, 3.1 pg/mL
for IL-2, 7.8 pg/mL for IL-4, 31.3 pg/mL for IL-10, 15.6 pg/mL for
tumor necrosis factor-, and 7.8 pg/mL for IL-12 p70.
Bone marrow transplantation Before transplantation, recipient mice were pretreated with either FL (10 µg/d) or diluent for 8 consecutive days (days 9 to
2). Mice then received transplants according to a standard protocol as described previously.21 Briefly, on day 0, mice received 12 to 13 Gy total body irradiation (TBI) (cesium Cs 137 source) split into 2 doses, separated by 3 hours to minimize
gastrointestinal toxicity. Then 5 × 106 BM cells and
2.5 × 106 nylon wool purified splenic T cells
resuspended in 0.25 mL were injected intravenously into recipients. For
analysis of cell division, nylon wool-purified splenic T cells were
labeled with carboxy fluorescein diacetate-succinimidyl ester (CFSE;
Molecular Probes, Eugene, OR) and were transferred into irradiated
recipients. In some experiments, BMT recipients were treated with 200 µg NK1.1 mAbs (clone PK134) on days 2 and 1 of BMT to eliminate
natural killer (NK) cells.22 Mice were housed in
sterilized micro-isolator cages; they received autoclaved
hyper-chlorinated drinking water for the first 3 weeks after BMT and
filtered water thereafter.
Systemic and histopathologic analysis of acute GVHD Survival after BMT was monitored daily, and the degree of clinical GVHD was assessed weekly by a scoring system that sums changes in 5 clinical parameters: weight loss, posture, activity, fur texture, and skin integrity (maximum index, 10) as previously described.23 This index is a more sensitive index of acute GVHD severity than weight loss alone, a parameter that has been found to be reliable indicator of systemic GVHD in multiple murine models. Acute GVHD was also assessed by detailed histopathologic analysis of liver, a primary GVHD target organ. Sections of liver (right lobe) were fixed in 10% buffered formalin. Specimens were then embedded in paraffin, cut into 5-µm-thick sections, and stained with hematoxylin and eosin for histologic examination. Slides were coded without reference to prior treatment and were examined systematically by a single pathologist using a semiquantitative scoring system as previously described.24Statistical analysis Survival curves were plotted using Kaplan-Meier estimates. The Mann-Whitney U test was used for the statistical analysis of in vitro data and clinical GVHD scores, whereas the Mantel-Cox log rank-test was used to analyze survival data. P < .05 was considered statistically significant.
FL administration preferentially expands resting DCs Mice were injected with 10µg FL or diluent for 8 days, and their splenocytes were analyzed by a flow cytometry. Mice treated with FL showed a 2.4-fold increase in overall cellularity in spleen with a dramatic 28.2-fold increase in the absolute number of CD11c+ major histocompatibility complex (MHC) class II+ cells (75.6 ± 15.5 × 106/spleen) (Figure 1). In addition, numbers of CD11b+ CD11c macrophages, B220+ B
cells, and NK1.1+ cells were increased by 5.0-, 2.8-, and
3.9-fold, respectively, as previously shown,4 though the
number of CD3+ cells was unaffected. To determine the
effects of FL on DC activation, splenic DCs were gated according to
forward versus side scatter and CD11c positivity, and their surface
antigen expression was analyzed by 2-color immunofluorescence. Freshly
isolated control DCs and FL DCs displayed a resting, nonactivated
phenotype, as evidenced by low levels of surface MHC class II, CD80,
and CD86 (Figure 2).
FL DCs are poor stimulators of allogeneic T cells We next compared FL DCs to control DCs as stimulators of T-cell responses in an allogeneic MLR. As shown in Figure 3A, FL DCs were less effective stimulators than control DCs throughout the culture period. Similar results were obtained at different T/DC ratios and in other allogeneic responder-stimulator combinations (data not shown). Levels of IL-2 and IFN-, critical cytokines secreted during allogeneic T-cell
responses, were also decreased in the supernatants of MLR cultures
stimulated with FL DCs (Figure 3B-C). Neither IL-4 nor IL-10 was
detected in any of the supernatants. Immature DCs can induce tolerance
by generating IL-10-producing regulatory T (Tr1) cells in an
IL-10-dependent fashion.25,26 Therefore, T cells from
IL-10/ mice were used as responders in MLR. However,
T-cell proliferation from IL-10/ mice and wild-type
mice were equally impaired in culture with FL DCs (data not shown),
ruling out IL-10 production by Tr1 cells as a mechanism for the lack
of response.
Allostimulatory activity of FL DCs remains impaired after maturation in culture To determine whether the impaired allostimulatory function of FL DCs was caused by the expansion of immature DCs, we examined the ability of overnight culture, which can drive maturation,27,28 to restore the allostimulatory capacity of FL DCs. Overnight culture induced comparable phenotypic maturation in FL DCs and control DCs as characterized by increased expression of MHC class II, CD80, and CD86 (Figure 4). This phenotypic maturation correlated with an increased ability of cultured control DCs to stimulate proliferation and cytokine secretion of allogeneic T cells in MLR (Figure 5, Figure 3). By contrast, cultured FL DCs remained poor stimulators of all allogeneic T-cell responses. Thus, the impaired allostimulatory function of FL DCs could not be explained by reduced expression of costimulatory molecules on their surfaces.
Because APCs can inactivate T cells with which they interact through a
veto function,29 we next tested FL DCs for such inhibitory activity by adding graded numbers of FL DCs to control DCs in an
allogeneic MLR. FL DCs did not inhibit the stimulation of allogeneic T
cells by control DCs, but they showed an additive stimulatory capacity,
ruling out possible veto activity (Figure
6).
FL preferentially expands CD8 + DC subset stimulates allogeneic T
cells less efficiently than CD8 DCs in MLR in
vitro,16-18 we next investigated the effect of FL administration on these DC subsets. As shown in Figure
7, FL preferentially expanded
CD8+ DCs. The number of CD8+ DCs
was 50.9 ± 7.4 × 106/spleen (46-fold higher than
control mice), and the number of CD8 DCs was
33.7 ± 19.3 × 106/spleen (19-fold higher than control
mice). The ratio of CD8+ to CD8 DCs
increased 3.0-fold (1.51 ± 0.74 vs 0.47 ± 0.06;
P < .01). CD8+ DCs express low levels of
CD11b on their surfaces in contrast to the high levels detected on
CD8 DCs.4,30 FL treatment also increased
the ratio of CD11b to CD11b+ DCs by 3.3-fold
(Figure 7), showing that the increase in CD8+ DC number
was not attributed to an isolated up-regulation of CD8 on the cell
surface but rather to an expansion of the CD8+ DC
subset. When stimulated with a combination of Staphylococcus aureus Cowan I and granulocyte macrophage-colony-stimulating
factor (as well as various combinations of cytokines including IFN- and IL-4), CD8+ DCs consistently produced 10-fold more
IL-12 p70 than CD8 DCs (data not shown), in agreement
with previously published reports.30-32
Comparative allostimulatory activity of sorted
CD8 + DCs
to CD8 DC subsets to stimulate the allogeneic T cells
in vitro. Freshly isolated control DCs and FL DCs were sorted according
to their CD8+ expression, and reanalysis of the sorted
cell populations confirmed greater than 98% purity of each subset. In
culture, freshly isolated CD8 DCs were more efficient
stimulators of allogeneic T cells than CD8+ DCs in MLR
(Figure 8A), as previously
described.16,17,33,34 Of importance, each subclass of FL
DCs and control DCs stimulated T-cell proliferation to an identical
degree (Figure 8A). Furthermore, when CD8+ and
CD8 fractions sorted from control DCs were mixed at
the same ratio as that found in splenocytes from mice treated with FL
(CD8+/CD8, 7:3), the allostimulatory
capacity of the control DC mixture was equivalent to the FL DC mixture
(Figure 8B). Similarly, when a ratio of CD8+ to
CD8 DCs in spleens from FL-treated mice was changed to
that found in control spleens, (CD8+/CD8a,
3:7), the allostimulatory capacity of the mixture was equivalent in
FL-treated DCs and controls. Similarly, IFN- and IL-2 production from MLRs using CD8 DCs was greater than that in
cultures using CD8+ DCs (Figure 8C-D). For all ratios at
which the CD8+ and CD8 fractions from
FL DCs or control DCs were compared, IFN- and IL-2 production were
identical in each treatment group. Neither IL-4 nor IL-10 was detected
in any supernatant. Thus, the impaired allostimulatory activity of FL
DCs in MLR was caused primarily by the increased numbers of
CD8+ DCs produced by FL administration.
Expansion of host-type DCs by the administration of FL inhibits early donor T cell expansion and activation during a GVH reaction In a final set of experiments, we investigated the in vivo relevance of these in vitro findings using a mouse model of GVHD, wherein host-derived DCs play a critical role. B6D2F1 (H-2b/d, CD45.2+) mice were pretreated with either FL (10 µg/d) or diluent for 8 consecutive days before allogeneic BMT (days9 to 2). On day 0, mice received
2.5 × 106 nylon wool-purified splenic T cells from
allogeneic B6.Ly-5a (H-2b, CD45.1+) donor mice
after 13 Gy TBI. Four days after TBI, host-derived DCs
(CD45.2+ CD11c+) were undetectable in spleens
of mice receiving control diluent, whereas 6.8 × 104 DCs
were detected in FL-treated recipients; by day 6, these DCs had
disappeared from the spleen. Donor T-cell (CD45.1+
CD3+) expansion was evaluated in spleens on day 3 after
transfer, when they responded to differences in MHC class I and MHC
class II and multiple minor histocompatibility antigens of the host. Despite the marked increase of DCs in recipients by the administration of FL before BMT, allogeneic donor T-cell expansion was almost completely ablated in FL-pretreated recipients on day 4 (Figure 9A). Analysis of cell division among
these cells using carboxy fluorescein diacetate-succinimidyl ester dye
showed lack of cell division correlating with this impaired donor
T-cell expansion (3.1 × 104 FL vs
50.9 × 104 control). In control recipients of allogeneic
T cells, T cell activation markers CD25 and CD49 appeared on donor
CD45.1+ CD3+ T cells on day 4 but were
dramatically suppressed in FL-pretreated mice (Figure 9B-C). As an
additional index of systemic T-cell responses in vivo, serum levels of
IFN- were measured on day 4, the time of peak concentration, and
were also significantly decreased in FL-pretreated mice (Figure 9D).
However, donor T-cell expansion in FL-treated mice did increase and
equaled that of control mice on day 7 after BMT (data not shown). Thus,
FL pretreatment of recipients inhibits early donor T-cell expansion and
activation to host alloantigens in vivo, which is critical for the
entire clinical course of acute GVHD.35,36
Pretreatment of hosts with FL reduces death from acute GVHD Donor T-cell expansion and activation after BMT normally result in severe systemic GVHD and death in this model system. B6D2F1 recipient mice were treated with either 8-day FL (10 µg/d, day9 to day 2)
or diluent and then were given 12 Gy TBI on day 0 and received
transplants of 5 × 106 BM cells and
2.5 × 106 nylon wool-purified splenic T cells from
B6.Ly-5a donors. GVHD was severe in controls, with 24% recipient
survival at day 60, whereas 68% of FL-pretreated recipients survived
(Figure 10A, P < .01).
Allogeneic control mice developed severe clinical GVHD compared with
syngeneic controls, as assessed by alterations in fur texture, skin
integrity, posture, mobility, and weight loss.23 These
signs were significantly less severe in FL-treated mice at all time
points compared to allogeneic controls (P < .05), though
scores in remained significantly higher than in syngeneic controls (Figure 10B). Weight loss as a single parameter of acute GVHD
was also less pronounced in FL-treated mice than in control mice at week 9 (20% ± 2% vs 32% ± 1%; P < .05).
Histopathologic examination of the liver on day 14 showed significantly
lower GVHD pathology scores in FL-treated animals (Figure 10C;
P < 0.05). Analysis of donor engraftment at day 60 after
BMT in peripheral blood showed complete donor engraftment in
FL-pretreated recipients (99.3% ± 0.7%), ruling out rejection or
mixed chimerism as a potential cause of reduced GVHD. FL treatment
before BMT thus, significantly reduced the ability of host APCs to
activate donor T cells and significantly attenuated, but did not
eliminate, acute GVHD.
FL treatment expands NK cells,37 and host NK cells play a
role in hybrid resistance in this strain combination.22 To
examine the in vivo effects of FL on host NK cells and GVHD, B6D2F1
mice received FL (10 µg/d, day
FL treatment of mice reduced their ability to stimulate allogeneic
T cells in MLR despite the fact that DC numbers increased and that
freshly isolated FL DCs and control DCs from spleens were in similarly
inactivated and resting states, as characterized by the low expression
of MHC class II and costimulatory molecules.11,38 This
observation is consistent with recent findings that demonstrate the
impaired allostimulatory capacity of DCs isolated from bone marrow of
FL-treated mice, though that study suggested that the impaired function
of FL DCs was probably a result of their immaturity.11 In
our experiments, however, FL DCs and control DCs displayed similar
phenotypes. Freshly isolated splenic DCs express little MHC class II,
CD80, or CD86, but these molecules are up-regulated in culture even
without any additional stimuli.27,28 Impaired functions of
FL DCs were not restored by the activation of FL DCs by overnight
culture in vitro. Thus, the allostimulatory function of FL DCs is
impaired regardless of their maturational status. Immature DCs can
induce tolerance by inducing Tr1 cells,25,26 but IL-10, a
critical cytokine secreted by Tr1 cells,25,26 was not
detected in the supernatant of MLR or in the serum of mice treated with
FL. FL DCs were also poor stimulators of IL-10 FL expanded splenic DCs primarily by increasing proliferation of
CD8 In vitro studies have suggested that CD8 We confirmed the importance of the decrease in allostimulation caused
by FL in vivo using a mouse model of GVHD in which the interaction of
donor-derived T cells with allogeneic host APCs plays a fundamental
role.42 Systemic administration of FL does not change the
distinct localization pattern of DC subsets: CD8 GVHD is a major cause of morbidity in BMT, and new approaches to this difficult problem are required. Efforts to prevent GVHD have long focused on the suppression of donor T-cell functions.43 Given the important role of host-derived APCs in GVHD induction, strategies to inactivate host DCs in BMT appear to be promising, though such novel selective targeting of APCs in vivo has not yet been clinically tested. We believe that these data represent the first demonstration of reduced GVHD by the modulation of host-derived DCs through the prophylactic administration of FL. This approach is unique because GVHD is ameliorated by the expansion rather than the elimination of host-derived DCs. The timing of FL administration within this strategy is critical, and our results stand in stark contrast to a recent report of the exacerbation of GVHD when recipients were given FL after BMT.44 One explanation for the difference between these studies is the lack of the effects of FL on host DCs in that study because host DCs essentially disappeared by day 6 after BMT. FL treatment did not expand DCs in that report, but it did up-regulate inflammatory cytokine expression. It is possible that macrophages-monocytes that were activated by TBI may be further stimulated by FL, and that could also increase the severity of GVHD. Recent evidence suggests that immature DCs and genetically engineered
DCs that constitutively express immunosuppressive molecules have the
potential to down-regulate immune responses.45 Our data
suggest a novel mechanism to modulate immune responses by the
administration of FL. This concept is also supported by a recent report
that donor-derived CD8 Our study showed that although FL treatment to recipients before BMT
significantly attenuated GVHD, it did not eliminate it. Perhaps the
impaired allostimulation by FL DCs is short lived because of an
extremely rapid turnover of CD8
Submitted August 2, 2001; accepted October 18, 2001.
Supported by National Institutes of Health grants CA39542 (J.L.M.F.) and HL03565-05 (K.C.).
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
Reprints: James L. M. Ferrara, Department of Internal Medicine, University of Michigan Cancer Center, 1500 E Medical Center Dr, Ann Arbor, MI 48109-0942; e-mail; ferrara{at}umich.edu.
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+ dendritic cells and
reduces experimental acute graft-versus-host disease
Top
Abstract
Introduction
friend or foe?
Immunity.
2001;14:357-368