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Infection and Immunity, April 2000, p. 2077-2081, Vol. 68, No. 4
Parasitology Research Center, Department of
Pathology, Tufts University Medical School, Boston, Massachusetts
Received 29 October 1999/Returned for modification 13 December
1999/Accepted 30 December 1999
Expression of functional transforming growth factor Trypanosoma cruzi is the
agent responsible for Chagas' disease, a chronic infection widespread
in Central and South America (4). T. cruzi is an
intracellular parasite in the mammalian host. Infectious metacyclic
trypomastigotes introduced in the feces of the hemophagic reduviid bug
invade host cells. Initially the parasite is located in a lysosomal
compartment, but it rapidly escapes into the cytoplasm. Amastigotes,
the intracellular form of the parasite, divide in the host cell
cytoplasm and then differentiate back into trypomastigotes, which are
released, destroying the cell and allowing continuation of infection in
new cells.
The process of mammalian cell invasion by T. cruzi and the
mechanisms of parasite survival within the host cell are poorly understood. Entry is accompanied by stimulation of several host cell
signaling pathways by trypomastigotes. Calcium transients (16), tyrosine phosphorylation (20), MAP kinase
activation (20), and transforming growth factor TGF- TGF- In order to study the role of TGF- Parasites and cells.
T. cruzi Silvio strain
trypomastigotes were maintained in Vero cells in RPMI medium
supplemented with 10% fetal bovine serum, 12.5 mM HEPES, 2 g of
sodium bicarbonate per liter, penicillin, and streptomycin (Gibco,
Rockville, Md.). Released trypomastigotes were harvested by
centrifugation at 500 × g for 5 min to remove host
cells and debris and at 1,200 × g for 10 min to
recover parasites. All experiments were carried out using wild-type
Mv1Lu or R4.2 cells, which are mutant Mv1Lu cells lacking functional
T Infection assays.
Mv1Lu cells were plated into 96-well
plates at 2 × 103/well and incubated overnight.
Expression of receptors or mutant SMAD proteins was induced by
replacement of medium with MEM containing 0.2% serum and 100 µM zinc
chloride and incubation for 4 to 6 h (17). For TGF- In order to determine the role of the growth arrest pathway in
infection with T. cruzi, R4.2 cells, whose T
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Copyright © 2000, American Society for Microbiology. All rights reserved.
Dual Role for Transforming Growth Factor
-Dependent Signaling in Trypanosoma cruzi Infection of
Mammalian Cells
ABSTRACT
Top
Abstract
Introduction
Materials and Methods
Results and Discussion
References
(TGF-)
receptors (TR) is required for the invasion of mammalian cells by
the protozoan parasite Trypanosoma cruzi. However, the
precise role of this host cell signaling complex in T. cruzi infection is unknown. To investigate the role of the
TGF- signaling pathway, infection levels were studied in the mink
lung epithelial cell lines JD1, JM2, and JM3. These cells express
inducible mutant TR1 proteins that cannot induce growth arrest in
response to TGF- but still transmit the signal for TGF--dependent
gene expression. In the absence of mutant receptor expression,
trypomastigotes invaded the cells at a low level. Induction of the
mutant receptors caused an increase in infection in all three cell
lines, showing that the requirement for TGF- signaling at invasion
can be divorced from TGF--induced growth arrest. TGF-
pretreatment of mink lung cells expressing wild-type TR1 caused a
marked enhancement of infection, but no enhancement was seen in JD1,
JM2, and JM3 cells, showing that the ability of TGF- to stimulate
infection is associated with growth arrest. Likewise, expression of
SMAD7 or SMAD2SA, inhibitors of TGF- signaling, did not block
infection by T. cruzi but did block the enhancement of
infection by TGF-. Taken together, these results show that there is
a dual role for TGF- signaling in T. cruzi infection.
The initial invasion of the host cell is independent of both
TGF--dependent gene expression and growth arrest, but TGF-
stimulation of infection requires a fully functional TGF- signaling pathway.
INTRODUCTION
Top
Abstract
Introduction
Materials and Methods
Results and Discussion
References
(TGF-) receptor (TR) activation (10) are all important
in invasion. The role of TGF- signaling in T. cruzi
infection is demonstrated by the fact that infection is very low in the
absence of TR1 or -2 and is restored by expression of the deficient
receptor (10). Preincubation of host cells with TGF-
causes a marked enhancement of infection (10), but the
mechanism by which TGF- promotes T. cruzi infection is
not known.
is a pleiotropic factor that regulates a number of cellular
functions and can stimulate expression of extracellular matrix
proteins, cell cycle arrest, cell growth, and apoptosis in different
cell types (15). The TR complex is made up of two
transmembrane serine/threonine kinases, TR1 and TR2
(21). TR2 kinase is constitutively active but cannot
induce signaling until TGF- binding induces association with TR1
(22). Phosphorylation of TR1 by TR2 activates kinase
activity and stimulates association with SMAD2 and SMAD3 (6, 9,
12). In unstimulated cells, these proteins are present in an
inactive form in the cytoplasm. Phosphorylation by TR1 activates
SMAD2 and SMAD3, causing association with the related protein SMAD4 and
translocation to the nucleus, where the SMAD complex binds to DNA and
triggers gene expression (1, 8, 9, 19). SMAD7, an inhibitory
member of the SMAD family, is induced by TGF- signaling (2,
13). This protein binds to TR1 and prevents association with
the signaling SMAD proteins, thereby blocking TGF- signaling.
signaling has been extensively studied by overexpression of
mutant receptors and SMAD proteins to dissect the function of different
components of the pathway. The mutant TR1 receptors, JD1, JM2, and
JM3, all contain mutations in the juxtamembrane region of the receptor
(17). JM2 and JM3 are mutated at specific phosphorylation
sites, Ser172 and Thr176, respectively, while JD1 lacks the entire
juxtamembrane region from amino acid 150 to 181. All three mutants are
active in kinase activity and can trigger changes in expression of the
matrix proteins fibronectin and plasminogen activator inhibitor, but
they cannot induce growth arrest. Overexpression of SMAD7 or of
SMAD2SA, a mutant of SMAD2 in which the phosphorylation sites (Ser465
and Ser247) are mutated to alanine residues, both block TGF-
signaling completely (1, 13, 19). Expression of SMAD2SD,
which contains aspartate residues in place of Ser465 and Ser467, leads
to constitutive activation of these pathways (19).
signaling in T. cruzi
infection, we utilized an inducible expression system in mink lung epithelial (Mv1Lu) cells to determine the effect of expression of
mutant TR1 proteins and SMAD family proteins on infection.
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials and Methods
Results and Discussion
References
R1. Stable transfectants of Mv1Lu and R4.2 cells were generated
with pMEP4-derived plasmids
pMEP4 expresses genes under the control of
the metallothionein promoter, which is activated by Zn2+
(17, 21). Construction of the plasmids and development of stable transfectants containing mutant TR1, SMAD2SA, and SMAD7 proteins are described in references 17, 19, and
7, respectively. Functional studies revealed that
the TR1 transfectants were resistant to growth arrest by 2 ng of
TGF-1 per ml, as described in references 7, 17,
and 19. Mv1Lu cells were maintained in minimal
essential medium (MEM) supplemented with nonessential amino acids, 10%
fetal bovine serum, 12.5 mM HEPES, 2 g of sodium bicarbonate per
liter, penicillin, and streptomycin (Gibco).
pretreatment, cells were incubated for 24 h in the presence of
various concentrations of recombinant human TGF-1 (R&D Systems,
Minneapolis, Minn.). For infection, trypomastigotes were added at a
concentration of 106/ml in RPMI medium-1% bovine serum
albumin for 2 h. The plates were washed with RPMI medium and then
incubated in MEM containing 2.5% Nu serum at 37°C for 48 h.
Plates were washed with phosphate-buffered saline and stained with
DiffQuik as described in reference 14. The percent
infection and number of parasites were determined for at least 300 cells per well. Significance was determined using Student's
t test.
RESULTS AND DISCUSSION
Top
Abstract
Introduction
Materials and Methods
Results and Discussion
References
R1 is
nonfunctional, were induced to express wild-type TR1 and mutant
TR1 proteins JD1, JM2, and JM3. The various transfectants were then
infected with T. cruzi trypomastigotes, and after 2 days,
the infection level in the cells was determined. Addition of 100 µM
zinc chloride had no significant effect on infection of wild-type Mv1Lu
(Fig. 1). R4.2 cells transfected with
pMEP4 alone show significantly lower levels of infection than wild-type
cells (P < 0.02). This is in accordance with the
observations made previously with the mutant Mv1Lu line R1B, which also
bears nonfunctional TR1 (10). The results with both R1B
and R4.2 cells show that T. cruzi requires functional TR1
expression for proper invasion, at least of epithelial cells.
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FIG. 1.
Expression of wild-type and mutant T R1 increases the
infection level in Mv1Lu cells. Wild-type (WT) Mv1Lu cells and R4.2
clone cells (bearing a mutated TR1 gene) were transfected with pMEP4
carrying wild-type TR1 or mutant receptors JD1, JM2, and JM3 and
incubated in the presence or absence of 100 µM ZnCl2 for
4 h prior to infection. Infection with Silvio strain
trypomastigotes was carried out as described in Materials and Methods.
Cells containing at least two amastigotes were scored as infected. At
least 300 cells were counted per well. Each bar represents the mean of
triplicate wells + the standard error of the mean. This graph is
representative of eight experiments with similar results.
No change in infection was seen when R4.2 cells were incubated with
zinc prior to infection. By contrast, the percentage of cells infected
was markedly increased in R4.2 cells transfected with pMEP4 carrying
the wild-type TR1 gene and exposed to zinc to induce receptor
expression, which is under the control of the zinc-sensitive
metallothionein promoter. Basal levels of infection in the
transfectants (i.e., in the absence of zinc stimulation) were also
higher in these cells, probably due to a low level of constitutive
receptor expression. Expression of the mutant receptors JD1, JM2, and
JM3 enhanced the infection level in each case. Consistent results were
obtained in eight experiments. These results show that expression of
TR1 is sufficient to enhance infection level, irrespective of the
ability of the receptor to induce growth arrest. Thus, although the
receptor is required for invasion, induction of growth arrest by the
parasite is unlikely to be the basis of that requirement.
Exposure of Mv1Lu cells to TGF- enhances infection dramatically
(10). To determine whether the growth arrest pathway might be involved in this enhancement, R4.2 cells expressing wild-type or
mutant receptors were incubated with various concentrations of TGF-
24 h before infection. In the absence of zinc, infection levels
were uniformly low in the presence or absence of TGF- (data not
shown). TGF- did not have any effect on infection of R4.2 cells
transfected with an empty plasmid (Fig.
2). Cells expressing wild-type TR1
showed a dose-dependent enhancement of infection with increasing
concentrations of TGF-1. However, in JD1, JM2, and JM3, the lines
expressing mutant TR1, TGF- had very little effect on the
infection level, either in terms of the percentage of cells infected
(Fig. 2A) or in terms of parasite replication (Fig. 2B). The ability of
TGF- to enhance infection is therefore closely associated with the
stimulation of growth arrest.
|
To determine the role of signaling events downstream of the TGF-1
receptor in T. cruzi infection, we employed Mv1Lu cells expressing two different mutant SMAD2 proteins, SMAD2SA and SMAD2SD, and SMAD7. SMAD2SA and SMAD7 are dominant negative inhibitors of
TGF- signaling, while SMAD2SD is constitutively active (13, 19). Like wild-type cells, Mv1Lu cells transfected with the plasmid pMEP4 alone showed similar levels of infection in the presence
and absence of zinc (Fig. 3). In cells
expressing SMAD2D, however, infection levels were significantly
enhanced (P < 0.01). The activation of signaling in
this case mimicked the effect of addition of exogenous TGF-1.
Interestingly, expression of either SMAD2SA or SMAD7 did not alter
infection. The two cell lines showed levels of infection similar to
that of the control cells transfected with pMEP4 alone, and addition of
zinc had no effect. Neither the number of cells infected nor the number
of parasites per cell (i.e., parasite replication) was affected by the
ectopic expression of SMAD2SA and SMAD7, suggesting that the SMAD
pathway has no direct involvement in infection of host cells by
T. cruzi.
|
To determine the role of the SMAD pathway in the stimulation of
infection by TGF-, cells were induced to express SMAD2SA or SMAD7
and then incubated with 2 ng of TGF-1 per ml prior to infection. In
the absence of zinc, TGF-1 pretreatment enhanced the percentage of
cells infected more than threefold (Fig.
4A). The effect on parasite replication
was even more dramatic (Fig. 4B). The levels of enhancement seen in
cells transfected with pMEP4 containing the SMAD2SA or SMAD7 gene were
similar to those in control cells transfected with pMEP4 alone. When
zinc was added to induce expression of either SMAD2SA or SMAD7, the
enhancement of infection by TGF- was partially, but not completely,
blocked (P < 0.01). This shows that the SMAD pathway
is involved in the enhancement of infection by TGF-, but it suggests
that other signals may also play a role.
|
The results presented here point to a dual role for TGF- signaling
in T. cruzi infection. The parasite requires receptor expression to enter host cells, but this requirement can be divorced from the downstream SMAD signaling pathway and from TGF--induced growth arrest. It has previously been shown that trypomastigotes can
trigger expression of genes controlled by TGF- and that
kinase-inactive TR1 does not support infection (10), but
in apparent contradiction, the major downstream signals induced by
TGF- do not seem to be very important in invasion. However, TR
expression is required for trypomastigote entry into the host cell,
rather than long-term establishment of infection (10).
Invasion is a rapid process, taking only a few minutes. Changes in gene
expression, while they may have an impact on parasite growth within the
host cell, are unlikely to contribute to parasite entry. It is more
likely that other yet-to-be-determined signals are involved as well in
T. cruzi invasion. TGF- has been shown to activate the
GTPase Ras (25), which is required for control of
transcription but not for growth arrest (24). TGF- also
activates the Rho family GTPases (3, 11, 24), which control
cell shape and motility (5). Other pathways stimulated by
TGF- include activation of kinases such as TAK1 (23),
SAPK (3), and Erk1 (11). These are early events
in TGF- signaling that may control infection. Other events, such as
receptor clustering and association with cytoplasmic proteins, could
also be important.
The role of TGF- itself in infection by T. cruzi is quite
distinct from the requirement for the TR. The enhancement of
infection is a long-term effect, closely associated with growth arrest
and at least partially dependent on the SMAD signaling pathway.
Previous work suggested that growth arrest per se is not sufficient to enhance infection (10). The effect of TGF- may therefore
depend on alterations in expression of specific genes during
TGF--induced growth arrest, rather than the growth arrest itself.
Although the role of exogenously added TGF- is distinct from the
role of parasite-induced receptor activation, the ability of TGF- to
enhance infection is highly relevant to parasite survival in vivo.
TGF--producing cells are abundant in heart lesions of mice infected
with T. cruzi (26). Infection of macrophages
induces TGF- expression, which in turn reduces the ability of gamma
interferon to control intracellular infection (18). In
addition, experimental T. cruzi infection is exacerbated by
injection of TGF-, showing that this cytokine is a key regulator of
infection (18). The presence of TGF- in infected tissues
serves to enhance infection directly by increasing susceptibility to
infection and indirectly by counteracting the effects of antiparasitic cytokines.
The dual role for the TGF- pathway in T. cruzi infection
demonstrates the importance of host cell responses in parasite
survival. Identification of the specific mechanisms underlying the two
effects may reveal novel aspects of TGF- signaling and lead to new
targets for the therapy of Chagas' disease.
| |
ACKNOWLEDGMENTS |
|---|
We thank P. ten Dijke, M. Saitoh. H. Ichijo, S. Souchelnytsky,
and S. Itoh for the stable transfectants of Mv1Lu containing TGF-.
This work was supported by NIH grant AI18102.
| |
FOOTNOTES |
|---|
* Corresponding author. Mailing address: Dept. of Pathology, Tufts University School of Medicine, 136 Harrison Ave., Boston, MA 02111. Phone: (617) 636-2933. Fax: (617) 636-6849. E-mail: Mpereira{at}infonet.tufts.edu.
Editor: W. A. Petri Jr.
| |
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Materials and Methods
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Copyright © 2000, American Society for Microbiology. All rights reserved.
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(2001). Borrelia burgdorferi-Induced Inflammation Facilitates Spirochete Adaptation and Variable Major Protein-Like Sequence Locus Recombination. J. Immunol.
167: 3383-3390
[Abstract] [Full Text]
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