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Previous Article | Next Article 
Infection and Immunity, February 2001, p. 665-672, Vol. 69, No. 2
Department of Pathology, College of
Veterinary Medicine and Biomedical Sciences, Colorado State
University, Fort Collins, Colorado 80523
Received 30 June 2000/Returned for modification 4 September
2000/Accepted 24 October 2000
The importance of CD40, CD80, and CD86 costimulatory molecules in
anti-Leishmania immune responses has been established in murine models. A role for these costimulatory molecules in human anti-Leishmania immune responses was investigated in this
study. Autologous macrophages and peripheral blood leukocytes (PBL)
were prepared from peripheral blood mononuclear cells of
Leishmania-naive donors and cultured with or without
Leishmania major in various combinations. After 7 days of
culture, high levels of CD40 and CD86 were expressed on macrophages in
the presence or absence of L. major. When macrophages were
cultured for an additional 7 days with PBL, expression of all three
costimulatory molecules was detected. When L. major was
present in these cultures, the expression of CD80, and to a lesser
extent CD40, on macrophages was enhanced. Blockade of CD80, CD86, or
both molecules (in the order of greatest effect) in cultures containing
macrophages, PBL, and L. major significantly inhibited the
production of gamma interferon, interleukin-5 (IL-5), and IL-12.
Blockade of CD40-CD154 interactions also significantly inhibited
production of these cytokines in response to L. major.
Production of IL-10 was unaltered by the blockade of these
costimulatory molecules. Thus, these data suggest that CD40, CD80, and
CD86 expression and regulation may significantly impact
anti-Leishmania immune responses in humans.
The outcome of experimental
cutaneous infection with Leishmania major in mice is
dependent on the strain of mouse and the predominating T-cell immune
response that develops. Resistance is associated with Th1 responses and
the appropriate production of interleukin-12 (IL-12) and gamma
interferon (IFN- Appropriate costimulation by CD40 may be essential for resistance in
Leishmania-infected mice, but an essential role for B7 costimulation is in dispute. In CD40- or CD154-deficient mice, impaired
production of IL-12 and IFN- With the exception of studies by Probst et al. (37),
showing up-regulation of CD80 on leishmanial antigen-treated human macrophages and dendritic cells, little is known of the role that costimulation plays in experimental human responses to
Leishmania infection. Based on what is known for mice, we
hypothesized that human responses to L. major would be
dependent on CD40 costimulation and influenced by both CD80 and CD86.
To test these hypotheses, we used an in vitro cell priming system (IVS)
for human peripheral blood mononuclear cells (PBMC) to investigate (i)
the influence of L. major infection on the expression of
these costimulatory molecules on macrophages in the presence or absence
of peripheral blood leukocytes (PBL) and (ii) the influence of CD40,
CD80, and CD86 costimulation on the production of Th1- and Th2-specific cytokines in response to L. major. We show that among these
molecules, CD86 and CD40 play a critical role in the initiation of
anti-Leishmania T-cell activation.
Parasites.
L. major (isolate LV39, R/SU/59/P)
parasites were grown on biphasic NNN medium (48) and
passed through mice every 2 weeks to maintain virulence. Stationary
metacyclic promastigotes were isolated by negative selection using
peanut agglutinin as described previously (38).
Reagents.
The following reagents were used in cell cultures:
human CTLA-4-Fc chimera (R&D Systems, Minneapolis, Minn.) at 10 µg/ml; neutralizing anti-human CD80 and CD86 monoclonal antibodies
(MAbs) (mouse immunoglobulin G1 [IgG1] isotype; R&D Systems) at 2.5 µg/ml; neutralizing anti-CD154 MAb (mouse IgG1 isotype; PharMingen,
San Diego, Calif.) at 10 µg/ml; and irrelevant isotype-matched
antibodies from the same suppliers, used as controls at the same
concentrations. The following reagents were used for flow cytometry:
fluorescein isothiocyanate (FITC)-labeled anti-human CD14 (clone TUK4,
mouse IgG2a; Caltag, Burlingame, Calif.); phycoerythrin (PE)-labeled anti-human CD80 (clone L307.4, mouse IgG1; PharMingen); PE- and FITC-labeled anti-human CD86 (clone 2331, mouse IgG1; PharMingen); CyChrome-labeled anti-human CD40 (clone 5C3, mouse IgG1; PharMingen); FITC-labeled anti human HLA DR, DP, and DQ (clone TU 39, mouse IgG2a;
PharMingen); and appropriately labeled irrelevant isotype-matched control antibodies from the same suppliers.
IVS.
Human blood was obtained from healthy individuals at
the Student Health Center of Colorado State University. Blood was
collected from each donor at two time points (stages 1 and 2), 7 days apart.
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.2.665-672.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Influence of Costimulatory Molecules on Immune
Response to Leishmania major by Human Cells In
Vitro
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
), leading to parasite destruction by macrophages
(33, 34, 39, 48). Susceptibility is associated with Th2
responses, early IL-4 production, IL-12 insensitivity, and a failure of
IFN--induced macrophage activation (7, 24, 29, 30).
Because costimulation of T cells by antigen-presenting cells (APCs;
e.g., dendritic cells and macrophages) has been shown to influence the
activation of T cells (18, 20), the influence of
costimulatory molecule expression in mice on their resistance to
Leishmania infection has been investigated.
is observed along with an increased
mortality rate following Leishmania infection (6, 26,
45). In contrast, in CD28-deficient strains of mice, both Leishmania-resistant and Leishmania-susceptible
phenotypes were maintained following infection (3),
suggesting that B7-CD28 costimulation played a limited role. However,
treatment of L. major-infected mice with CTLA-4Ig caused
normally susceptible mice to develop protective Th1 responses
(9), suggesting that B7 costimulation is essential for
susceptibility. This inference was supported by results in the same
study showing that CTLA-4Ig had no effect on the outcome of infection
in normally resistant mice. More recently, blockade of CD86, but not
CD80, in susceptible mice was shown to decrease parasite burdens and
the production of Th2 cytokines following L. major infection
(4). These results suggested that CD86, and not CD80, is
critical for Th2 differentiation. However, other studies have indicated
that B7 costimulation is required for the early development of both
resistant and susceptible anti-Leishmania responses in mice,
and that CD86 functions as the dominant costimulatory molecule in both
cases (12). Thus, the role of B7 costimulation in
experimental leishmaniasis is unclear.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
20°C until assayed.
In stage 3, secondary stimulation of PBL blasts was performed. The
blast cells obtained in stage 2 were washed and resuspended in complete
medium at 4 × 106 cells/ml. These cells were
restimulated by culturing (1 ml/well) for 48 h at 37°C with 5%
CO2 with the autologous Leishmania-infected adherent cells obtained in stage 2. No blocking reagents were added to
these cultures. Culture supernatants were collected and stored at
20°C until assayed.
Cytokine assays.
Concentrations of IFN-, IL-5, IL-10, and
IL-12 in culture supernatants were determined by enzyme-linked
immunosorbent assay (ELISA) using commercial anticytokine antibody
pairs (PharMingen) and a protocol provided by the manufacturer. Human
recombinant IFN-, IL-5, IL-10, and IL-12 (PharMingen) were used to
generate standard curves. The limits of detection for these assays were 10 pg/ml for IFN-, IL-10, and IL-12 and 2 pg/ml for IL-5.
Flow cytometry.
Monocytes and macrophages were analyzed for
costimulatory molecule expression. Monocytes were obtained as fresh
PBMC and were identified by expression of CD14. Macrophages were
obtained from cultures of adherent cells (see "IVS" above) by using
tissue culture cell scrapers (resultant cells were 
90% viable by
trypan blue exclusion) and were identified by their expression of MHC
class II. Cells (5 × 105/sample) were prepared for
analysis by resuspension in PAB (phosphate-buffered saline, 1% bovine
serum albumin, 0.05% sodium azide) and blocked with mouse Ig (20 µg/ml) and 10% fetal bovine serum for 30 min on ice. Cells were then
incubated with labeled antibodies or corresponding controls for an
additional 30 min. Cells were fixed with 1% paraformaldehyde in
phosphate-buffered saline and analyzed on a Coulter XL flow cytometer
(Coulter Corp., Hialeah, Fla.).
Statistical analysis. Comparison of cytokine levels between treatment groups and across multiple experiments was done by analysis of variance two-way ANOVA followed by Tukey all-ways comparison posthoc t tests. All tests were performed with Sigma-Stat software (SPSS Inc., Chicago, Ill.). Differences were considered significant at P < 0.05.
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RESULTS |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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Expression of costimulatory molecules on monocytes/macrophages in
the presence or absence of L. major and PBL.
Freshly
isolated CD14+ monocytes and cultured MHC class
II+ macrophages were analyzed for expression of CD40, CD80,
and CD86 molecules. As shown in Fig. 1A to
C, each of these molecules was expressed
on some CD14+ monocytes; whereas few monocytes expressed
CD80 (2% [Fig. 1A]) and CD40 (4% [Fig. 1C]), 70% expressed CD86
(Fig. 1B). Expression of costimulatory molecules was also observed on
some MHC class II+ macrophages after 7 days of culture
(Fig. 1D to F). Few macrophages expressed CD80, and then only at low
levels (Fig. 1D), whereas most (70%) expressed CD86 (Fig. 1E). The
expression of both CD80 and CD86 on macrophages was similar to that
observed on monocytes (see above). In contrast to monocytes,
approximately half (53%) of the macrophages expressed CD40 (Fig. 1F).
The presence of L. major during the last 24 h of
culture did not alter the expression of CD80 or CD40 on macrophages
(Fig. 1D and F). Compared with unexposed macrophages, the expression of
CD86 on L. major-exposed macrophages was only slightly
reduced, if changed at all (Fig. 1E), and only on macrophages from some
donors (data not shown).
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Blockade of costimulatory molecules alters L. major-specific cytokine production. Because costimulatory molecules can influence Th1 and Th2 cytokine production, and because L. major was shown to alter costimulatory molecule expression on macrophages cultured in the presence of PBL (see above), we examined the relative importance of CD40, CD80, and CD86 expression on the production of cytokines associated with Th1 and Th2 responses. PBL were stimulated with L. major-infected macrophages in (i) primary cultures with or without blocking reagents and (ii) secondary cultures without blocking reagents (stages 2 and 3 of IVS [see Materials and Methods]).
CD40-CD154 blockade.
The influence of CD40 expression on
L. major-specific cytokine production was examined by
blocking CD40-CD154 interactions with anti-CD154. As shown in Fig.
2, the presence of anti-CD154 during
primary stimulation of PBL resulted in significantly reduced IFN-
(Fig. 2A) and IL-5 (Fig. 2B) levels compared to cultures containing
isotype-matched control antibody. This difference in cytokine levels
was also observed following blast cell restimulation even though no
anti-CD154 was present in these cultures (Fig. 2C and D).
Interestingly, no change in IL-10 levels was detected in primary (Fig.
3A) or secondary (data not shown)
cultures as a result of anti-CD154 exposure, whereas anti-CD154
exposure reduced the amount of IL-12 to undetectable levels in both
primary (Fig. 3B) and secondary (data not shown) cultures.
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CD80 and/or CD86 blockade.
The influence of CD80 and CD86
expression on L. major-specific cytokine production was
examined by blocking B7-CD28 and B7-CTLA-4 interactions with CTLA-4Ig.
As shown in Table 1, the presence of
CTLA-4Ig during primary stimulation of PBL resulted in the reduction of
IFN- and IL-5 to below detectable levels. Cytokine levels in
cultures containing control Ig were comparable to those seen in
previous control cultures (see above) and cultures containing no
control reagent (Table 1). The reduction of cytokine levels resulting
from CTLA-4Ig exposure in primary cultures persisted in cultures of
restimulated blast cells (Table 1). To investigate the contribution of
individual B7 subtypes to cytokine production, we blocked
CD80/CD86-CD28 and CD80/CD86-CTLA-4 interactions with anti-CD80 and
anti-CD86 antibodies. As shown in Fig. 4,
the presence of anti-CD80 during primary stimulation of PBL resulted in
a slight but nonsignificant reduction of IFN- (Fig. 4A) and IL-5
(Fig. 4B) levels compared to cultures containing isotype-matched
control antibody. The presence of anti-CD86 significantly reduced both IFN- and IL-5 levels, an effect that was greater than that observed for anti-CD80 exposure. The presence of both anti-CD80 and anti-CD86 during primary stimulation led to a significant and near-complete elimination of detectable cytokine levels (Fig. 4A and B,
respectively), results similar to those obtained when CTLA-4Ig was
used. Similar reductions of IFN- and IL-5 levels resulting from
anti-CD80 and anti-CD86 exposure persisted in cultures of restimulated
blast cells and were similarly statistically significant (Fig. 4C and D). No consistent effect of anti-CD80 or anti-CD86 on IL-10 levels was
detected in primary (Fig. 5A) or
secondary (data not shown) cultures. However, a slight but increasingly
significant decrease in IL-12 levels resulting from exposure to
anti-CD80, anti-CD86, or both antibodies, similar to that seen for
IFN- and IL-5, was observed in both primary (Fig. 5B) and secondary
(data not shown) cultures.
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DISCUSSION |
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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The importance of various costimulatory molecules (e.g., CD40, CD80, and CD86) to the outcome of disease following Leishmania infection of mice has been examined. CD40 has been associated with resistance (6, 22, 26, 45), whereas the role of CD80 and CD86 is unclear (3, 4, 9, 12). Infection of mouse macrophages can alter costimulatory molecule expression, at least in vitro (27, 36, 41, 49). However, the impact on host resistance, if any, of this potential subversion of immune function is unclear. Although evidence suggests that dendritic cells play the major role in priming antileishmanial responses (31, 49), macrophages too are host cells for Leishmania and play the major role in killing these parasites (33, 34, 48). This parasitocidal activity is likely dependent, in part, on the macrophage's interaction with T cells (35). Little is known of the role that costimulation plays in directing anti-Leishmania responses in humans. Therefore, we undertook the study presented here to examine (i) the influence of L. major on costimulatory molecule expression on human monocyte-derived macrophages and (ii) the interactions of these macrophages with L. major-activated T cells.
Because costimulatory molecule expression has been shown to be modulated on nonhuman APCs following Leishmania infection in vitro (27, 36, 41, 49), we first determined if the expression of these molecules on cultured human macrophages was modulated following infection with L. major. CD86 expression was slightly decreased by L. major infection, but this effect was not observed with all donors, and we found no change in the expression of CD40 or CD80 (Fig. 1). Thus, no marked alteration of costimulatory molecule expression was observed on L. major-infected human macrophages. These results are similar to those for C57BL/6 mouse macrophages: no change in CD80 expression was observed following infection with L. donovani (41), and no change in CD40, CD80 or CD86 expression was observed following infection with L. major (49). However, Leishmania-induced changes in expression of costimulatory molecules has been observed on macrophages from BALB/c mice and dogs: decreased CD80 expression was observed following infection with L. donovani (27, 41) and L. infantum (36), respectively. From a comparison of the results shown here for humans, and shown by others in animal models, it seems reasonable to predict that the sensitivity of macrophages to modulation of costimulatory molecule expression following Leishmania infection may be dependent on the host's genetic background.
Because T cells may interact directly with infected macrophages through
costimulatory molecules to promote parasite killing (35),
we also examined the influence of T cells on the expression of
costimulatory molecules by L. major-infected and uninfected macrophages. Infection with L. major had no effect on CD86
expression by macrophages cocultured with PBL (Fig. 1). In contrast,
coculture with PBL led to an increase in CD40 and CD80 expression on
L. major-infected macrophages (Fig. 1). These findings are
significant because they demonstrate the feedback interactions between
APCs and effector cells and suggest that the effects of L. major on macrophages, at least in part, require such interactions.
These interactions may include indirect mechanisms, such as IFN-,
which is known to induce expression of CD80 and to up-regulate
expression of CD86 on monocytes (11, 14), or direct
mechanisms such as stimulation of CD40 by CD154, which has been shown
to up-regulate both CD40 and CD86 (28). A combination of
direct and indirect mechanisms seems likely in this system.
This is the first report that live L. major modulates costimulatory molecule expression on human macrophages, but it is not the first such report regarding intracellular parasites. For example, Subauste et al. observed that infection of human monocytes with tachyzoites of Trypanosoma gondii caused a rapid induction of CD80 expression and up-regulation of CD86 (46). On the other hand, infection of mouse macrophages with L. donovani or Mycobacterium tuberculosis failed to up-regulate or actually decreased the expression of CD80 and CD86 (27, 40). These effects on costimulatory molecule expression may represent strategies used by pathogens to induce anergy or otherwise cause advantageous immune suppression. Interestingly, the results presented here contrast with those of Probst et al. (37), who cultured human macrophages (without PBL) in the presence of a purified Leishmania protein, LeIF, and showed an increase in both CD40 and CD80 expression. This difference in results may be due to confounding interactions between the multitude of potentially immunomodulatory factors released by live parasites versus a single purified protein, or a difference in the concentrations of LeIF present in the macrophage cultures.
We had predicted that primary human responses to L. major
would be dependent on CD40 costimulation and influenced by CD80 and
CD86 costimulation. These predictions were shown to be mostly true.
Blocking CD40 or CD86 significantly reduced the production of IFN-,
IL-12, and IL-5 following stimulation with L. major, whereas
the only significant effect of blocking CD80 was a reduction in IL-12
production. Thus, of these three costimulatory molecules, CD40 and CD86
played the greatest role in initiating human in vitro anti-L.
major responses. The relatively small influence of CD80 in this
system is an interesting finding in light of the marked up-regulation
of CD80 on macrophages cultured with PBL and L. major. The
mechanism(s) behind this lack of effect is unclear, but a low
sensitivity to CD80 costimulation may be a characteristic of PBMC, as
suggested by others (2, 23).
Our prediction that CD40 would be essential to human in vitro responses
to L. major was based on well-established pathways: (i) CD40
ligation leads to IL-12 production which leads to IFN- production
and (ii) CD40 induces up-regulation of B7 molecules on APCs (for
reviews, see references 15 and 18). Thus, our finding that blocking CD40 ligation reduced IL-12 and IFN-
production is not unique to anti-Leishmania responses, but
it is important to know that in human cells, as in mouse cells,
L. major does not alter the predictability of this
costimulatory pathway. The greater effect of CD40 blockade over B7
blockade could be explained, in part, by a double effect on cytokines
and B7 expression when CD40 ligation was inhibited.
An unexpected observation was the reduction of IL-5 production in macrophage+L. major+PBL cultures following blockade of CD40 and CD86. IL-5 was used as an indicator of Th2 cell activity. The importance of CD40 to the development of Th1 responses has been well established, but the role of this costimulatory pathway in the development of Th2 responses is less well studied. The results of the studies presented here suggest that CD40, as well as CD86, can costimulate for both Th1 and Th2 responses. Similar findings in another model (44, 47) suggest that, at least for CD40, this may be a common phenomenon.
As shown here, IL-10 production was not significantly altered by
blocking CD40 or the B7 molecules, unlike what was observed for IL-5,
IL-12, and IFN-. The IL-10 levels measured in these studies were
lower than those observed by others following mitogen or MAb
stimulation (5, 10, 43) and were more in line with spontaneous production levels (5, 25). This can be
explained by the use of metacyclic L. major in the study
presented here. Metacyclic L. major has been shown to be a
poor stimulator of IL-10 production from human PBMC, unlike the
log-phase promastigote form of the parasite (42). Because
blocking costimulation did not alter IL-10 levels, these results
suggest that spontaneous or metacyclic L. major-stimulated
IL-10 production is independent of the costimulatory molecules
examined. Others have shown that IL-10 production can be modulated by
IL-12 and IFN- (1, 8, 10, 15). Therefore, it was
interesting that IL-10 levels were not changed in the face of markedly
lower IL-12 and IFN- levels. These data suggest that spontaneous or
metacyclic L. major-stimulated IL-10 production is also
independent of modulation by IL-12 and IFN-. This possibility is
supported for IL-12 by the results of Sartori et al. (42),
who showed that IL-10 production by metacyclic L. major-infected human PBMC was unchanged by treatment with
anti-IL-12 MAb.
In summary, we showed that L. major infection can influence the expression of some costimulatory molecules on human macrophages, with the greatest effect apparent in the presence of PBL. Further, we showed that CD40 and CD86 play critical roles in the initiation of human anti-Leishmania T-cell activation in vitro.
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ACKNOWLEDGMENTS |
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We thank Robin Morris for technical assistance and Lamine Mbow critical review of the manuscript.
This work was supported by NIH grant AI-29955 and a fellowship (to C.I.B.) from CAPES/Fulbright (1997) and CAPES-Brasilia Brazil (1998).
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FOOTNOTES |
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* Corresponding author. Mailing address: Department of Pathology, College of Veterinary Medicine and Biomedical Sciences, Colorado State University, Fort Collins, CO 80523. Phone: (970) 491-4964. Fax: (970) 491-0603. E-mail: rtitus{at}cvmbs.colostate.edu.
Present address: Laboratório de Imunologia, Departamento de
Biointeração, Instituto de Ciências da Saúde,
Universidade Federal da Bahia, Salvador, Bahia, Brazil.
Editor: W. A. Petri Jr.
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Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
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) and means (bars) are presented with background cytokine
levels subtracted. Background equaled the concentration of cytokine
when PBL were stimulated with uninfected adherent cells and ranged <10
to 270 pg/ml for IFN-
