![[Feedback]](/icons/banner/feedbackACT.gif){kind=icon}
![[For Subscribers]](/icons/banner/subscriberACT.gif){kind=icon}
![[Archive]](/icons/banner/archiveACT.gif){kind=icon}
![[Search]](/icons/banner/searchACT.gif){kind=icon}
![[Contents]](/icons/banner/tocACT.gif){kind=icon}
Previous Article | Next Article 
Infection and Immunity, September 2001, p. 5270-5277, Vol. 69, No. 9
Instituto Butantan, São
Paulo,1 and Medical School of
Itajubá, Minas Gerais,3 Brazil;
Infectious Disease Research
Institute2 and Corixa
Corporation,4 Seattle, Washington 98104;
and Immunex Corporation, Seattle, Washington
981015
Received 7 March 2001/Returned for modification 2 May 2001/Accepted 20 June 2001
The interaction of the innate immune system with the microbial
world involves primarily two sets of molecules generally known as
microbial pattern recognition receptors and microbial pattern recognition molecules, respectively. Examples of the former are the
Toll receptors present particularly in macrophages and dendritic cells.
Conversely, the microbial pattern recognition molecules are conserved
protist homopolymers, such as bacterial lipopolysaccharides, lipoteichoic acids, peptidoglycans, glucans, mannans, unmethylated bacterial DNA, and double-strand viral RNA. However, for protists that
lack most of these molecules, such as protozoans, the innate immune
system must have evolved receptors that recognize other groups of
microbial molecules. Here we present evidence that a highly purified
protein encoded by a Leishmania brasiliensis gene may be
one such molecule. This recombinant leishmanial molecule, a homologue
of eukaryotic ribosomal elongation and initiation factor 4a (LeIF),
strongly stimulates spleen cells from severe combined immunodeficient
(SCID) mice to produce interleukin-12 (IL-12), IL-18, and high levels
of gamma interferon. In addition, LeIF potentiates the cytotoxic
activity of the NK cells of these animals. Because LeIF is a conserved
molecule and because SCID mice lack T and B lymphocytes but have a
normal innate immune system (normal reticuloendothelial system and NK
cells), these results suggest that proteins may also be included as
microbial pattern recognition molecules. The nature of the receptor
involved in this innate recognition is unknown. However, it is possible to exclude the Toll receptor Tlr4 as a putative LeIF receptor because
the gene encoding this receptor is defective in C3H/HeJ mice, the mouse
strain used in the present studies.
Stimulation of the immune system by
most microorganisms is usually carried out by molecules that interact
with two distinct sets of host recognition molecules, namely, the
microbial pattern recognition receptors and the antigen receptors of T
and B lymphocytes (6, 7). These receptors are responsible
for the initiation and expression of the innate and adaptive immune
responses, respectively. Microbial pattern recognition receptors are
germ line encoded, and it is estimated that their repertoire is
restricted to a few hundred different receptors (12). In
contrast, T and B lymphocyte antigen receptors are generated by somatic
genetic mechanisms and their repertoires are on the order of
approximately 1015 different specificities
(2).
In general, the immune response is initiated by the recognition of the
microbial pattern recognition molecules by host cells. This results in
activation of the host cells to both produce several different
cytokines involved in the inflammatory reaction and present antigenic
epitopes to the highly specialized cognitive elements of the immune
system. While the latter elements can recognize practically all sorts
of foreign organic molecules, in particular, carbohydrates and
proteins, the elements involved in the pattern recognition molecules
are not as diversified. It is believed that the recognition repertoire
of this system is limited to bacterial lipopolysaccharides (LPS),
lipoteichoic acids, peptidoglycans, glucans, mannans,
bacterial DNA, and double-stranded viral RNA (12).
Although these molecules are chemically distinct from one another, they
have some properties in common; e.g., they all are homopolymers, and
with the exception of the nucleic acids, they are integral components
of the bacterial and fungal cell walls and are therefore limited to
these organisms of the microbial world. In addition, the
immune-regulatory properties of nucleic acids are primarily associated
with bacterial and viral DNA and RNA, respectively.
However, for microbes, such as protozoans, that lack cell walls and
have nucleic acids that are weaker stimulatory molecules than the
bacterial and viral counterparts (21), the vertebrate hosts must have evolved and developed receptor molecules that are
capable of recognizing different microbial molecules to alert the
innate immune system to subsequently initiate the specific immune response.
We have recently shown that a protozoan (Leishmania
brasiliensis) gene homologous to eukaryotic ribosomal elongation
and initiation factor 4A encodes a protein designated LeIF that
stimulates peripheral blood mononuclear cells (PBMC) from both
leishmaniasis patients and uninfected individuals (22,
23). Stimulation of these cells, as well as normal human
monocyte-derived macrophages and dendritic cells, with LeIF resulted in
the production of large quantities of gamma interferon (IFN- To investigate this possibility, we used severe combined
immunodeficient (SCID) mouse spleen cells because these mice lack mature T and B lymphocytes but have functional macrophages and NK
cells, essential components of the innate immune system. The results
confirm and expand our former observation, in that LeIF activates
macrophages to produce IL-12 and IL-18 and NK cells to produce IFN- Animals.
SCID mice in the LPS low-responder genetic
background (C3H/HeJ) aged 6 to 8 weeks were obtained from The Jackson
Laboratory and maintained at our facilities in specific-pathogen-free condition.
Reagents.
Recombinant mouse IL-12 and polyclonal sheep
anti-murine IL-12 were kindly supplied by the Immunology Department of
the Genetic Institute (Cambridge, Mass.). Recombinant human IL-15 and
IL-2, murine granulocyte-macrophage colony-stimulating factor, and IL-4 were provided by Immunex Corp. (Seattle, Wash.). Recombinant mouse IL-5
and IFN-
0019-9567/01/$04.00+0 DOI: 10.1128/IAI.69.9.5270-5277.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.
Potent Stimulation of the Innate Immune System by a
Leishmania brasiliensis Recombinant Protein
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
) and
interleukin-12 (IL-12) p40 and p70 (18). Therefore, LeIF
could be a microbial protein recognized by the elements of the innate
immune system. However, because in these experiments we could not rule
out the possibility that LeIF was recognized by contaminating T cells,
i.e., by cognitive receptors, it became important to test if LeIF would
stimulate the innate components of immunity in the absence of the
cognitive elements of the immune system.
.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
were from Pharmingen (San Diego, Calif.), and recombinant IL-18 was purchased from Pepro Tech, Inc. (Rocky Hill, N.J.). Purified
anti-mouse IL-5 and IFN- monoclonal antibodies (MAbs) were from
Pharmingen. Rabbit anti-asialo GM1 antiserum was purchased from Wako
Chemicals (Dallas, Tex.). Purified anti-tumor necrosis factor alpha,
anti-mouse CD11b (Mac-1), anti-CD80 (B7.1), anti-CD86 (B7.2), and
anti-mouse CD32/16 were purchased from Pharmingen. LPS was purchased
from Sigma Chemical Co. (St. Louis, Mo.). LeIF was prepared as
previously described (22), followed by reverse-phase high-pressure liquid chromatography using a gradient of
acetonitrile in water (both eluants contained 0.05% trifluoroacetic
acid). Pure fractions were pooled and lyophilized before being
redissolved in Tris buffer (10 mM, pH 8.0) prior to use. Figure
1 illustrates the high degree of purity
of the protein used in these studies. Purified leishmanial recombinant
proteins 8E and Ldp23 and mycobacterial recombinant proteins TbH9 and
TbRa1 were provided by Corixa Corporation (Seattle, Wash.). All
recombinant proteins contained less than 10 ng of endotoxin per mg of
protein, as determined by the Limulus amoebocytelysate (LAL)
assay.
View larger version (12K):
[in a new window]
FIG. 1.
High-pressure liquid chromatography profile of
purified LeIF. Au, arbitrary units.
Cell preparation.
Spleens from C3H/HeJ SCID mice were
removed aseptically and dissociated in RPMI medium containing 10%
fetal bovine serum, 50 µM 2 
-mercaptoethanol, and 50 µg
of gentamicin per ml. Single-cell suspensions were prepared after lyses
of red blood cells with ammonium chloride. After two washes, the cells
were counted and plated in 96-well flat-bottom plates at a density of 2 × 105/100 µl of RPMI 1640 medium. Bone
marrow-derived macrophages were obtained from the bone marrow of
C3H/HeJ SCID mice by Ficoll gradient, washed twice with RPMI
1640 medium, and plated in six-well plates at a density of
5 × 106 to 8 × 106 cells per well
in 5 ml of RPMI 1640 medium. After 2 h at 37°C, the
nonadherent cells were removed and the cultures were submitted to
another overnight adherent cycle of purification. The adherent cells
were cultured in RPMI 1640 medium plus 20 ng each of recombinant murine
granulocyte-macrophage colony-stimulating factor and recombinant murine
IL-4 per ml. Every 3 days, the cells were fed with fresh supplemented
medium. After 8 to 12 days, the cells were harvested for assay. The
cells were analyzed by FACScan cytoflurometer using the Cell Quest
software (Becton Dickinson) and shown to be 98% MAC-1-positive cells.
, B7.1/B7.2, and
asialo-GM+.
Cytotoxicity assays.
The specific cytotoxic activity of
activated spleen cells against 51Cr-labeled YAC-1 target
cells was measured in a standard 4-h chromium release assay at several
effector-to-target ratios. Percent specific 51Cr release
was calculated by using the following formula: (experimental release 
spontaneous release)/(maximum release spontaneous release) × 100. Spontaneous release was obtained from target cells in the
absence of effector cells, and maximum release was obtained by lysis of
target cells with Triton X-100. The results are expressed as the mean
of triplicate wells of one representative experiment from at least
three identical experiments.
Cytofluorometric analysis. The expression of cell surface markers was performed by standard procedures on a FACSCalibur (Becton Dickinson). The following fluorescein isothiocyanate-labeled antibodies, purchased from Pharmingen, were used for staining: anti-CD11b (MAC-1), anti-CD80 (B7-1), anti-CD86 (B7-2), and anti-CD14. Purified anti-mouse CD32/CD16 was used to block the nonspecific binding of MAbs to Fc receptors. For NK cell staining, spleen cells or activated NK cells were incubated with a 1/250 dilution of polyclonal rabbit anti-asialo-GM1 serum for 30 min at 4°C. Background fluorescence was assessed by using normal rabbit serum. Cells were washed and then incubated with biotinylated anti-rat immunoglobulin G, followed by incubation with phycoerythrin-conjugated streptavidin for 30 min at 4°C. Stained cells were analyzed by FACS.
ELISA.
The two-site enzyme-linked immunosorbent assay
(ELISA) was employed to assay the levels of IFN-, IL-5, and IL-12.
Briefly, 96-well plates were coated overnight at 4°C with 2 µg of
either anti-murine IL-5 (TRFK5), IL-12 (C.17.15.10.12), or anti-IFN- (R4-6A2) MAbs per ml in bicarbonate buffer, washed with
phosphate-buffered saline-0.05% Tween 20 (Sigma Chemical Co., St.
Louis, Mo.), and blocked with phosphate-buffered saline-1% bovine
serum albumin for 2 h. After washing, samples were added and
incubated overnight at 4°C. Plates were washed, followed by the
addition of biotinylated anti-mouse IL-5 (TRFK4), anti-mouse IL-12
(C.15.6.7.6), or anti-mouse IFN- (XMG1.2) MAbs at 0.5 mg/ml, and
incubated for 2 h at room temperature. The plates were washed and
incubated for an additional 1 h with streptavidin-peroxidase.
After the last washing, the reactions were developed with
tetramethylbenzidine (TMB) substrate and read at 450 nm.
| |
RESULTS |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
IFN- production by SCID spleen cells stimulated with LeIF.
We have previously shown that PBMC from leishmaniasis patients and
normal donors produce IFN- in response to LeIF (22). However, the mechanism by which LeIF elicits this IFN- production was not systematically investigated. Three types of cells produce IFN-, CD4+ Th1 lymphocytes, CD8+ T
lymphocytes, and NK cells. To investigate the requirement, or lack
thereof, of T-cell recognition for the production of IFN- by normal
cells stimulated with LeIF, spleen cells from T-cell deficient SCID
mice were used. SCID mice lack mature T and B cells, and their spleens
are highly enriched with NK cells (3, 4, 8, 11).
Therefore, this is an ideal system with which to test the action of
LeIF in the absence of specific immune recognition. Cells were
activated with different concentrations of LeIF for 48 to 72 h,
and the cytokine concentration was analyzed in the culture
supernatants. The results shown in Fig.
2A indicate that LeIF stimulates resting
NK cells in a dose-dependent manner for the production of high levels
of IFN-. This effect was not due to LPS contamination because the
LeIF preparations used in these studies contained less than 10 ng of
endotoxin per mg of protein (LAL assay). In addition, the LPS inhibitor
polymyxin B had little or no effect on LeIF-induced IFN- production
by SCID spleen cells. In contrast, polymyxin B inhibited LPS-induced
IFN- production by these cells by >90% (Fig. 2B). Moreover,
treatment of LeIF with proteinase K totally abolished its activity
(data not shown).
|
production by NK
cells, such as IL-12 and IL-18, LeIF induced greater quantities of
IFN- than either IL-12 or IL-18, even when these inflammatory
cytokines were used at high concentrations (10 U/ml and 100 ng/ml,
respectively). In addition, IL-15, which is a cytokine that stimulates
NK cells to proliferate via components of IL-2R, did not stimulate SCID
mouse spleen cells to produce IFN-. Interestingly, LeIF induced high
levels of IFN- production in the absence of a significant
proliferative response of the SCID spleen cells (Fig.
3).
|
was due to
LeIF or if the His tag portion of the recombinant protein induced this
activity. To test this possibility, several recombinant proteins (with
a His tag in the N terminus) from different origins, including two
proteins from other species of Leishmania and two from
Mycobacterium tuberculosis, were compared with LeIF. The
results indicate that LeIF was the only microbial recombinant protein
to induce IFN- production in SCID spleen cells. None of the other
His tag recombinant protein tested stimulated these cells (data not shown).
Characterization of SCID spleen cells that interact with LeIF for
production of IFN-.
Because the only cell population capable of
producing IFN- in the SCID mouse spleen is NK cells, it became
interesting to determine if LeIF stimulates these cells directly or
indirectly, for example, via cytokines produced by activated
macrophages. To investigate this possibility, a direct approach was
initially used. NK cells were purified from SCID spleen cells after
removal of macrophages and other adherent cells by two passages over
Sephadex G-10 columns. The purified (enriched) NK cells were stimulated with either LeIF or IL-15. No IFN- could be detected in the
supernatant of these cultures (Fig 4A).
However, excellent proliferation was obtained when these cells were
stimulated with IL-15, thus confirming their viability after the two
passages over Sephadex G-10 columns (data not shown). To dissect
further the cells involved in the induction by LeIF of IFN-
production by SCID spleen cells, a lymphokine-activated NK cell line
(LAK) devoid of antigen-presenting cells was generated. This LAK cell
line was obtained after several cycles of stimulation of
macrophage-depleted (with Sephadex G-10 column) SCID spleen cells
with IL-15. FACS analysis revealed the following cell surface pattern:
CD14, B7.1/B7.2, and
asialo-GM1+ (data not shown). Stimulation of these
highly purified NK cells with LeIF again resulted in no production of
IFN-. However, when bone marrow macrophages were added to the
purified NK or to the LAK cells, great quantities of this cytokine were
produced by both cell populations (Fig. 4). No IFN- was detected in
the culture supernatants of bone marrow macrophages alone either
incubated with medium or in the presence of LeIF (data not
shown). These results indicate first that LeIF does not act
directly on the NK cells and second that its ability to stimulate
IFN- production by these cells is dependent on antigen-presenting
cells.
|
Characterization of the cytokines involved in the
LeIF-stimulated macrophages necessary for IFN- production by NK
cells.
One of the most intriguing characteristics of LeIF is its
strong ability to induce both human PBMC and PBMC-derived macrophages to produce IL-12 (18, 22). Because this cytokine and
IL-18, another macrophage-derived cytokine, are actively involved in the activation of both T cells and NK cells for the production of
IFN- (13, 15, 25), we investigated the participation of
these cytokines in IFN- production by SCID mouse spleen cells stimulated with LeIF. Cells were stimulated with LeIF in the presence or in the absence of rabbit anti-IL-12 or rabbit anti-IL-18 antibody for 72 h. Supernatants were harvested and analyzed for the
presence of IFN-. Figure 5 clearly
shows that both antisera inhibited IFN- production by
LeIF-stimulated SCID mouse spleen cells. Because IL-12 acts
synergistically with IL-18 to induce IFN- production by T cells
(10, 13, 24), these results strongly suggest that the
potent activation of SCID mouse spleen cells by LeIF for the production
of IFN- is caused by the activation of macrophages and/or dendritic
cells to secrete both IL-1 and IL-18.
|
per ml,
respectively. In contrast, the addition of 10 µg of LeIF per ml to
these cultures resulted in the production of 63, 86, and 96.9 ng of
IFN- per ml, respectively (Fig. 6). The same pattern of synergistic response became even more evident when
exogenous IL-18 was used instead of IL-12. When the intrinsic ability
of IL-18 alone to induce the production of IFN- was compared with
that of its combination with LeIF, the results were striking. Undetectable or little IFN- production (less than 1 ng/ml) was obtained when SCID spleen cell cultures are stimulated with 4 to 100 ng
of IL-18 per ml alone. In contrast, up 654 ng of IFN- per ml was
obtained when 10 µg of LeIF per ml was added to these cultures (Fig.
6).
|
Stimulation of NK cell cytotoxicity by LeIF.
Because
LeIF-stimulated SCID spleen cells result in IL-12- and IL-18-dependent
production of high levels of IFN- by NK cells, we next investigate
if this stimulation would also result in the activation of the
cytolytic pathway of these cells. In these experiments, SCID spleen
cells were stimulated for 24 h with LeIF alone or in combination
with either IL-12 or IL-18. NK cell cytolytic activity was measured by
a standard 51Cr release assay using YAC-1 cells as targets.
Figure 7 illustrates the results. As can
be seen, LeIF alone caused an increase in the cytolytic activity of the
NK cells. In contrast, little or no killing activity was observed when
NK cells were stimulated with either IL-12 or IL-18 alone. However, an
excellent synergistic effect was observed when these two cytokines were
used to stimulate NK cells. Moreover, LeIF could substitute for either
one of these cytokines to achieve strong activation of killing activity
by NK cells. These results confirm that, like the activation of NK cells for IFN- production, LeIF induces the lytic activity of these
cells indirectly, i.e., via the stimulation of both IL-12 and IL-18 by
SCID mouse spleen cells.
|
Stimulation of SCID mice by LeIF leads to selective activation of a
distinct subset of NK cells.
Stimulation of lymphoid cells from
both leishmania-infected humans and mice with LeIF results in the
preferential production of Th1 cytokines (18, 22, 23). In
addition, LeIF stimulates normal human monocyte-derived cells to
produce IL-12. In order to investigate the pattern of cytokine
stimulation by LeIF in the absence of T-cell recognition, SCID mouse
spleen cells were stimulated with LeIF and the production of both
IFN- and IL-5 in the culture supernatants was determined by ELISA.
IFN- and IL-5 have been shown to be produced by distinct subsets of
NK cells, namely, NK1 and NK2, respectively (16). Because
IL-5 is a Th2 cytokine, it is believed that activation of NK2 cells could be associated with the Th2 pattern of immune response during the
innate phase of activation of the immune system. The results shown
in Fig. 8 clearly point to the production
of only IFN- by SCID spleen cells stimulated with various
concentrations of LeIF. No IL-5 could be detected in the supernatants
of these cells. In contrast, when the spleen cells were stimulated
with phorbol myristate acetate (PMA) and ionomycin, both
IFN- and IL-5 were produced, indicating that both the NK1
and NK2 cell subsets were activated after polyclonal stimulation.
|
| |
DISCUSSION |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
The innate immune system is activated by several microbial homopolymers usually associated with microorganisms' cell walls. In addition, bacterial DNA and double-stranded viral RNA are also potent activators of this system. These microbial homopolymers have been generally referred to as pathogen-associated molecular patterns and are widely distributed in the protist kingdom. However, higher protists, such as protozoans, lack cell walls and their nucleic acids activate the immune system to a lesser extent than do bacterial DNA and viral RNA (21). Therefore, recognition of these organisms by the host innate immune system must be done by alternative stimulating molecules.
LeIF, a recombinant protein encoded by an L. brasiliensis
gene, may be one such molecule. The gene that encodes it is present in
all members of the Leishmania genus thus far analyzed, and the protein is expressed in both the promastigote and amastigote forms
of these parasites. LeIF induces human PBMC from either leishmaniasis
patients or normal individuals to produce IL-12 and IFN- production
(22). In addition, LeIF induces the production of IL-12 by
monocyte-derived macrophages and dendritic cells (18). Therefore, LeIF could be a microbial molecule capable of alerting the
innate immune system to initiate an immune response.
In the present study, we investigated the ability of LeIF to activate
the innate immune system under a stringent condition, i.e., in the
total absence of the cognitive elements of the immune system. These
studies were carried out with cells from SCID mice because these
animals lack mature T and B cells and their spleens have a normal
reticuloendothelial system and are highly enriched with NK cells
(3, 4, 8, 11). They are therefore ideal for investigation
of the activation of the noncognitive elements of the immune system.
Our results demonstrated that naive SCID mouse spleen cells stimulated
with LeIF produced IL-12, IL-18, and high levels of IFN- in a
dose-dependent manner. This response was clearly not due to possible
contamination of LeIF with LPS because this activity was resistant to
polymyxin B and because the levels of LPS present in the preparation of
LeIF used in these studies were below the sensitivity of the LAL assay.
Compared with other recombinant proteins from leishmania or M. tuberculosis, LeIF was revealed to be a unique microbial protein that is able to induce NK cells to produce IFN- because only LeIF,
and none of the proteins tested, stimulated NK cells.
Studies designed to elucidate the mechanisms of action of LeIF
indicated that this molecule stimulates NK cells indirectly. This
conclusion was drawn based on the following experiments: First, removal
of macrophages from SCID mouse spleen cells totally abrogated the
ability of LeIF to stimulate the macrophage-depleted cells to produce
IFN-. Likewise, macrophage-free NK cell lines generated from SCID
mouse spleen cells by using IL-15 did not produce IFN- upon
stimulation with LeIF or IL-15, despite extensive proliferation in
response to the latter stimulus. However, reconstitution of these cells
with bone marrow-derived macrophages completely restored the ability of
these cells to produce large quantities of IFN- upon stimulation
with LeIF.
These experiments also led to the characterization of the molecular
events triggered by LeIF for the activation of NK cells. Because we
have shown earlier (18, 22, 23) that LeIF stimulates human
macrophages and dendritic cells to produce IL-12 and IL-18, these
cytokines became prime candidates to explain the LeIF stimulation of
murine NK cells to produce IFN-. Indeed, inhibition experiments using either anti-IL-12 or IL-18 antibodies clearly demonstrated that
both cytokine are responsible for the LeIF activation of SCID mouse
spleen cells for the production of IFN-. Moreover, it appears that
LeIF stimulates the right balance and physiological levels of these
cytokines by macrophages. This possibility is supported by the
experiments designed to evaluate the synergism between these two
cytokines. These experiments revealed that the levels of added
exogenous IL-12 or IL-18 necessary for optimal production of IFN- by
SCID spleen cells were much higher than the levels of both IL-12 and
IL-18 produced by the SCID macrophages upon stimulation with LeIF.
Curiously, the levels of IL-12 and IL-18 induced by LeIF in the culture
supernatants were below the sensitivity of the ELISA used in these
studies. Only mRNAs for both cytokines could be detected in
LeIF-stimulated cells (data not shown).
One possible explanation for these findings is that LeIF, in addition
to inducing the production of the cytokines themselves, also induces
up-regulation of the IL-12 and IL-18 receptors on NK cells. This
possibility is supported by the experiments that showed that addition
of either exogenous IL-12 or exogenous IL-18 to SCID mouse spleen cells
stimulated with LeIF resulted in an exceptional synergistic effect in
the form of a level of IFN- production not achieved by the addition
of the two cytokines together in the absence of LeIF. Experiments to
address this possibility are in progress. Alternatively, it is possible
that LeIF induces other factors that might act synergistically with
IL-12 or IL-18.
The production of very high levels of IFN- by LeIF-stimulated SCID
mouse spleen cells may be attributed to the absence of T cells in SCID
mice and consequently to the lack of regulatory cytokines produced by
these cells, such as, for example, IL-10. Indeed, LeIF, in addition to
inducing IL-12, also induces the production of IL-10 by both human and
conventional mouse cells (18). However, no IL-10 could be
detected in cultures of LeIF-activated SCID mouse spleen cells (data
not shown). Because IL-10 is a well-known inhibitor of IFN-
production, this observation could explain the abundant production of
IFN- by LeIF-stimulated SCID mouse spleen cells in this study.
Recent studies have demonstrated that stimulation of NK cells can cause
up-regulation of CD28 (14). In addition, it has been
proposed that the interaction of CD28+ NK cells with
B7+ accessory cells is an important asset in the control of
infections like those caused by Toxoplasma gondii
(5). In the present studies, the participation of these
costimulatory molecules on the activation of NK cells by LeIF was
investigated. FACS analysis revealed up-regulation of B7.1 but not of
B7.2 after 36 h of stimulation of SCID mouse spleen cells with
LeIF. However, addition of anti-B7.1 and anti-B7.2 during the
activation of NK cells with LeIF did not interfere with the ability of
NK cells to produce IFN- (data not shown). These results suggest
that the interaction of CD28, B7.1, and B7.2 does not participate in
the LeIF activation of NK cells for the production of IFN-.
Compared to the potent activation of NK cells for the production of
IFN-, the killing activity of these cells was stimulated to a lesser
extent by LeIF alone. However, after the exogenous addition of IL-12 or
IL-18, LeIF appreciably augmented the killing activity of NK cells.
These results suggest that the signals involved in signal transduction
mechanisms for the production of cytokines, particularly IFN-, and
cytotoxicity are not the same in NK cells.
Also interesting was the observation that LeIF stimulated the
generation of only the NK1 response phenotype in SCID mouse spleen
cells. In contrast, the polyclonal activators PMA and ionomycin stimulated both the NK1 and NK2 phenotypes. These results are apparently the first to expand to mice the former observation with
human cells suggesting that NK cells can differentiate into cells of
two phenotypes similar to those described for T cells. The
production of large amounts of IFN- and undetectable levels of IL-5
in LeIF-stimulated cells could be a determining factor in the
Th1-biased immune response to this molecule that is observed in
both human and mouse cells. However, because NK cells do not produce
IL-4 (9) and IL-5 is not implicated in the generation of
Th2 responses, one cannot directly correlate the activation of the two
subsets of NK cells as determinant factors in the generation of the two
subsets of cytokine-producing T cells (Th1 and Th2).
We do not have any information on a possible unique physical or chemical characteristic(s) of the LeIF molecule that could explain its biological properties. LeIF is a polypeptide comprised of 403 amino acids with a predicted molecular mass of 45.3 kDa and an isoelectric point of 5.9. The molecule contains 46 strongly basic amino acids, 55 strongly acidic amino acids, 91 polar amino acids, and 148 hydrophobic amino acids. A Kyte-Doolittle hydrophilicity plot suggests that the molecule has no major clusters of hydrophobic amino acids. LeIF is a cytoplasmic (ribosomal) protein involved in the translation machinery. The molecule contains sequence elements characteristic of several demonstrated or putative ATP-dependent RNA helicases represented by eukaryotic initiation factor 4A, which is believed to be a relatively abundant protein. Moreover, LeIF is present in both the promastigote and amastigote parasite forms of all of the Leishmania species thus far tested, as revealed by both Northern and Western blot analyses (22). Indeed, we have cloned, expressed, and analyzed the L. major homologue of L. brasiliensis LeIF. At the protein level, these two molecules have 99.8% homology and 98.3% total homology. In addition, we have determined that the biological activity of LeIF resides in the N-terminal half of the molecule (23). Unfortunately, we have been unable to purify the native form of LeIF to homogeneity and to unquestionably attribute to the native molecule the biological properties of the recombinant protein.
In conclusion, we report here that a recombinant protein obtained from
L. brasiliensis is a powerful stimulator of SCID mouse spleen cells for the production of IL-12, IL-18, and IFN- in the
absence of the cognitive recognition elements of the immune system.
Because of this property and because LeIF does not fit the classical
pathogen-associated molecular patterns, this work points to an
important finding, i.e., the description of alternative microbial
components (proteins) that alert the host to the presence of an
infecting or foreign organism. Incidentally, protein molecules extracted from other protozoans, such as T. gondii, and from
Trypanosoma cruzi have been reported to stimulate
mononuclear cells from noninfected mice to produce IL-12 and other
inflammatory cytokines (1, 20). The nature of the possible
cell receptor involved in the activation of the innate immune system by
LeIF is not known and is currently under investigation. It is possible,
however, to exclude the recently described Toll receptor Tlr4 as a
putative LeIF receptor because the gene encoding this receptor is
defective with a loss-of-function mutation in C3H/HeJ mice (17,
19), the mouse strain used in the present studies.
| |
ACKNOWLEDGMENTS |
|---|
We thank Thomas Vedvick for performing N-terminal sequencing and Pamela J. Ovendale for excellent technical assistance.
This work was supported by National Institutes of Health grant AI25038.
| |
FOOTNOTES |
|---|
* Corresponding author. Mailing address: Infectious Disease Research Institute, 1124 Columbia St., Suite 600, Seattle, WA 98104. Phone: (206) 381-0883. Fax: (206) 381-3678. E-mail: acampos{at}idri.org.
Editor: J. M. Mansfield
| |
REFERENCES |
|---|
|
Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References
|
|---|
| 1. | Almeida, I. C., M. M. Camargo, D. O. Procopio, L. S. Silva, A. Mehlert, L. R. Travassos, R. T. Gazzinelli, and M. A. Ferguson. 2000. Highly purified glycosylphosphatidylinositols from Trypanosoma cruzi are potent proinflammatory agents. EMBO J. 19:1476-1485[CrossRef][Medline]. |
| 2. | Davis, M. M., and P. J. Bjorkman. 1988. T-cell antigen receptor genes and T-cell recognition. Nature 334:395-402[CrossRef][Medline]. (Erratum, 335:744, 1988.) |
| 3. | Dorshkind, K., G. M. Keller, R. A. Phillips, R. G. Miller, G. C. Bosma, M. O'Toole, and M. J. Bosma. 1984. Functional status of cells from lymphoid and myeloid tissues in mice with severe combined immunodeficiency disease. J. Immunol. 132:1804-1808[Abstract]. |
| 4. | Garni-Wagner, B. A., P. L. Witte, M. M. Tutt, W. A. Kuziel, P. W. Tucker, M. Bennett, and V. Kumar. 1990. Natural killer cells in the thymus. Studies in mice with severe combined immune deficiency. J. Immunol. 144:796-803[Abstract]. |
| 5. | Hunter, C. A., L. Ellis-Neyer, K. E. Gabriel, M. K. Kennedy, K. H. Grabstein, P. S. Linsley, and J. S. Remington. 1997. The role of the CD28/B7 interaction in the regulation of NK cell responses during infection with Toxoplasma gondii. J. Immunol. 158:2285-2293[Abstract]. |
| 6. | Janeway, C. A., Jr. 1989. Approaching the asymptote? Evolution and revolution in immunology. Cold Spring Harbor Symp. Quant. Biol. 54:1-13. |
| 7. | Janeway, C. A., Jr. 1992. The immune system evolved to discriminate infectious nonself from noninfectious self. Immunol. Today 13:11-16[CrossRef][Medline]. |
| 8. | Kumar, V., J. Hackett, Jr., M. M. Tutt, B. A. Garni-Wagner, W. A. Kuziel, P. W. Tucker, and M. Bennett. 1989. Natural killer cells and their precursors in mice with severe combined immunodeficiency. Curr. Top. Microbiol. Immunol. 152:47-52[Medline]. |
| 9. |
Lauwerys, B. R.,
N. Garot,
J. C. Renauld, and F. A. Houssiau.
2000.
Cytokine production and killer activity of NK/T-NK cells derived with IL-2, IL-15, or the combination of IL-12 and IL-18.
J. Immunol.
165:1847-1853 |
| 10. | Lauwerys, B. R., J. C. Renauld, and F. A. Houssiau. 1999. Synergistic proliferation and activation of natural killer cells by interleukin 12 and interleukin 18. Cytokine 11:822-830[CrossRef][Medline]. |
| 11. |
Lauzon, R. J.,
K. A. Siminovitch,
G. M. Fulop,
R. A. Phillips, and J. C. Roder.
1986.
An expanded population of natural killer cells in mice with severe combined immunodeficiency (SCID) lack rearrangement and expression of T cell receptor genes.
J. Exp. Med.
164:1797-1802 |
| 12. |
Medzhitov, R., and C. Janeway.
2000.
Innate immunity.
N. Engl. J. Med.
343:338-344 |
| 13. |
Micallef, M. J.,
T. Tanimoto,
K. Kohno,
M. Ikeda, and M. Kurimoto.
1997.
Interleukin 18 induces the sequential activation of natural killer cells and cytotoxic T lymphocytes to protect syngeneic mice from transplantation with Meth A sarcoma.
Cancer Res.
57:4557-4563 |
| 14. | Nandi, D., J. A. Gross, and J. P. Allison. 1994. CD28-mediated costimulation is necessary for optimal proliferation of murine NK cells. J. Immunol. 152:3361-3369[Abstract]. |
| 15. | Okamura, H., S. Kashiwamura, H. Tsutsui, T. Yoshimoto, and K. Nakanishi. 1998. Regulation of interferon-gamma production by IL-12 and IL-18. Curr. Opin. Immunol. 10:259-264[CrossRef][Medline]. |
| 16. |
Peritt, D.,
S. Robertson,
G. Gri,
L. Showe,
M. Aste-Amezaga, and G. Trinchieri.
1998.
Differentiation of human NK cells into NK1 and NK2 subsets.
J. Immunol.
161:5821-5824 |
| 17. |
Poltorak, A.,
X. He,
I. Smirnova,
M. Y. Liu,
C. V. Huffel,
X. Du,
D. Birdwell,
E. Alejos,
M. Silva,
C. Galanos,
M. Freudenberg,
P. Ricciardi-Castagnoli,
B. Layton, and B. Beutler.
1998.
Defective LPS signaling in C3H/HeJ and C57BL/10ScCr mice: mutations in Tlr4 gene.
Science
282:2085-2088 |
| 18. | Probst, P., Y. A. Skeiky, M. Steeves, A. Gervassi, K. H. Grabstein, and S. G. Reed. 1997. A Leishmania protein that modulates interleukin (IL)-12, IL-10 and tumor necrosis factor-alpha production and expression of B7-1 in human monocyte-derived antigen-presenting cells. Eur. J. Immunol. 27:2634-2642[Medline]. |
| 19. |
Qureshi, S. T.,
L. Lariviere,
G. Leveque,
S. Clermont,
K. J. Moore,
P. Gros, and D. Malo.
1999.
Endotoxin-tolerant mice have mutations in Toll-like receptor 4 (Tlr4).
J. Exp. Med.
189:615-625 |
| 20. | Sher, A., I. P. Oswald, S. Hieny, and R. T. Gazzinelli. 1993. Toxoplasma gondii induces a T-independent IFN-gamma response in natural killer cells that requires both adherent accessory cells and tumor necrosis factor-alpha. J. Immunol. 150:3982-3989[Abstract]. |
| 21. |
Shoda, L. K.,
K. A. Kegerreis,
C. E. Suarez,
I. Roditi,
R. S. Corral,
G. M. Bertot,
J. Norimine, and W. C. Brown.
2001.
DNA from protozoan parasites Babesia bovis, Trypanosoma cruzi, and T. brucei is mitogenic for B lymphocytes and stimulates macrophage expression of interleukin-12, tumor necrosis factor alpha, and nitric oxide.
Infect. Immun.
69:2162-2171 |
| 22. |
Skeiky, Y. A.,
J. A. Guderian,
D. R. Benson,
O. Bacelar,
E. M. Carvalho,
M. Kubin,
R. Badaro,
G. Trinchieri, and S. G. Reed.
1995.
A recombinant leishmania antigen that stimulates human peripheral blood mononuclear cells to express a Th1-type cytokine profile and to produce interleukin 12.
J. Exp. Med.
181:1527-1537 |
| 23. |
Skeiky, Y. A.,
M. Kennedy,
D. Kaufman,
M. M. Borges,
J. A. Guderian,
J. K. Scholler,
P. J. Ovendale,
K. S. Picha,
P. J. Morrissey,
K. H. Grabstein,
A. Campos-Neto, and S. G. Reed.
1998.
LeIF: a recombinant Leishmania protein that induces an IL-12-mediated Th1 cytokine profile.
J. Immunol.
161:6171-6179 |
| 24. |
Tominaga, K.,
T. Yoshimoto,
K. Torigoe,
M. Kurimoto,
K. Matsui,
T. Hada,
H. Okamura, and K. Nakanishi.
2000.
IL-12 synergizes with IL-18 or IL-1beta for IFN-gamma production from human T cells.
Int. Immunol.
12:151-160 |
| 25. |
Tomura, M.,
X. Y. Zhou,
S. Maruo,
H. J. Ahn,
T. Hamaoka,
H. Okamura,
K. Nakanishi,
T. Tanimoto,
M. Kurimoto, and H. Fujiwara.
1998.
A critical role for IL-18 in the proliferation and activation of NK1.1+ CD3 cells.
J. Immunol.
160:4738-4746 |
This article has been cited by other articles:
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
| J. Bacteriol. | J. Virol. | Eukaryot. Cell |
|---|
| Microbiol. Mol. Biol. Rev. | Clin. Vaccine Immunol. | All ASM Journals |
|---|
