Vol. 277, Issue 6, R1741-R1748, December 1999
PGE2 suppresses mitogen-induced Ca2+
mobilization in T cells
Mashkoor A.
Choudhry1,
Philip
E.
Hockberger2, and
Mohammed M.
Sayeed1
1 Trauma/Critical Care Research
Laboratories, Departments of Surgery and Physiology, Burn & Shock
Trauma Institute, Loyola University Chicago Medical Center, Maywood
60153; and 2 Department of
Physiology, Northwestern University Medical School, Chicago, Illinois
60611
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ABSTRACT |
PGE2-mediated suppression
of T cell proliferation during sepsis could result from altered
Ca2+ signaling. The present study
evaluated the effects of PGE2 on Ca2+ release from intracellular
stores and its influx through the plasma membrane in splenic T cells
from Sprague-Dawley rats. Intracellular Ca2+ concentration
([Ca2+]i)
responses in individual T cells were assessed using the
Ca2+ imaging technique, and the
release of Ca2+ from intracellular stores and
Ca2+ influx were spectrofluorometrically quantified in T
cell suspensions. Under unstimulated conditions, nearly 85% of T cells
exhibited [Ca2+]i
50 nM. After stimulation with concanavalin A (Con A), an increase in
[Ca2+]i
was recorded in ~60% of the cells. The pretreatment of T cells with
PGE2 had no apparent effect on
[Ca2+]i
in resting cells; it significantly suppressed the Con A-induced increase in
[Ca2+]i
in all of the Con A-responsive cells.
Ca2+ release from the
intracellular stores contributed to the early spike in
[Ca2+]i,
and the late phase of elevation in
[Ca2+]i
was dependent on Ca2+ influx
through the plasma membrane. Our data suggest that
PGE2 causes an overall suppression
of the Con A-induced
[Ca2+]i
elevation in T cells via inhibiting both
Ca2+ influx and its release from
the intracellular stores.
concanavalin A; T lymphocytes; calcium ion signaling; intracellular
calcium ion release; adenosine 3,5-cyclic monophosphate; prostaglandin
E2
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INTRODUCTION |
T CELL ACTIVATION and interleukin (IL)-2 production are
essential for appropriate functioning of the immune system (1, 2, 35).
The activation of T cells is effected primarily via stimulation of T
cell antigen receptor (TCR). Two of the TCR polypeptide chains forming
a heterodimer are important in recognizing the antigen; the others,
collectively called CD3, are involved in receptor assembly and signal
transmission (2, 36). The stimulation of TCR, in vivo, results from its
interactions with antigen-presenting cells (1, 2, 35, 36). In vitro,
TCR stimulation could be achieved with lectins or specific antibodies
directed against the CD3 complex (1, 2, 36) and gives rise to a series of intracellular responses eventually leading to T cell IL-2 production (1, 2, 4, 12, 35, 36). The intracellular responses include the
activation of protein tyrosine kinases and phospholipase C-
(1, 2,
4) with subsequent hydrolysis of phosphatidylinositol 4,5-bisphosphate
(PIP2) into inositol
1,4,5-trisphosphate (IP3) and
1,2-diacylglycerol. The
IP3-mediated release of
Ca2+ from intracellular stores is
followed by Ca2+ influx through
the plasma membrane causing a sustained elevation in intracellular
Ca2+ concentration
([Ca2+]i;
see Refs. 1, 2, 4, 5, 12, 14, 37). The increase in
[Ca2+]i
sustained for several hours is considered critical for T cell activation and IL-2 production (2, 4, 5, 21, 37).
An increased production and release of
PGE2 after burn and septic
injuries has been correlated with a decrease in T cell IL-2 production
and proliferation (8, 18, 20, 33). The role of
PGE2 in the suppression of T cell
IL-2 production and proliferation is borne out by direct effects of
PGE2 on T cells (6, 7, 24, 26, 28,
34). In previous studies, we showed that
PGE2-mediated suppression of T
cell functions is associated with an attenuation in T cell
Ca2+ signaling as assessed in T
cell suspensions (8, 10).
In the present study, we evaluated the effects of
PGE2 on
[Ca2+]i
responses in individual T cells using the
Ca2+ imaging technique. These
assessments allowed us to ascertain variability in the
[Ca2+]i
responses within the T cell population. We examined also the effects of
PGE2 on release of
Ca2+ from intracellular stores and
its influx through the plasma membrane. Additionally, we ascertained
the effect of intracellular cAMP, the second messenger generated in the
action of PGE2, in the modulation of T cell
[Ca2+]i
(3, 17, 23, 34).
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EXPERIMENTAL PROCEDURES |
Animals and reagents. Male
Sprague-Dawley rats (200-225 g) were obtained from Harlan Sprague
Dawley (Indianapolis, IN). PGE2, dibutyryl-cAMP (DBcAMP), EGTA, and concanavalin A (Con A) were purchased from Sigma Chemical (St. Louis, MO). Fura 2-AM was purchased from Molecular Probes (Eugene, Oregon). Thapsigargin was obtained from
Calbiochem-Novabiochem International (San Diego, CA). Ficoll-Paque and
nylon wool fiber were obtained, respectively, from Pharmacia Sweden and
Polysciences (Warrington, PA). All other cell culture reagents were
purchased from GIBCO-BRL (Grand Island, NY).
T cell preparation. Anesthetized rats
were killed, and their spleens were removed. Spleens were minced to
dissociate cells, and suspensions of single cells were prepared in
Hanks' balanced salt solution (HBSS). Red blood cells present in these
cell suspensions were removed using Ficoll-Paque. For the enrichment of
T cells, splenocytes were passed through a nylon wool column
preequilibrated with HBSS containing 10 mM HEPES, 5% FCS,
and 50 µg/ml gentamicin. After 45-60 min of incubation
of the columns with cells at 37°C, T cells were obtained by eluting
the columns with 20-25 ml of warm HBSS. Details of the T cell
preparation procedure have been reported previously (8, 10, 11).
Measurements of single cell
[Ca2+]i
using Ca2+
imaging.
T cell suspensions were loaded with 10 µM fura 2-AM for 1 h at room
temperature as described earlier (8, 10). Approximately 100 µl of the
cell suspension were placed on a coverslip and examined under a
×40 objective of an inverted microscope (Nikon). The cells were
exposed to alternating 340- and 380-nm excitation wavelengths, and
emission of fura 2 was collected through a 505-nm band-pass filter.
Images were obtained using a cooled-CCD-Camera (Sensys; Photometrics)
and image acquisition system (Universal Imaging). Images were corrected
for background fluorescence, separated into to ratios, and analyzed
using Metafluor software (Universal Imaging; see Ref. 25).
[Ca2+]i
was estimated by calibrating the imaging system with mixtures of
solutions of known Ca2+ and fura 2 concentrations (27).
Fluorometric measurements of
[Ca2+]i
in T cell suspension.
Fura 2-loaded cells were transferred to a cuvette, and fluorescence
signals were recorded using a Hitachi Spectrophotofluorometer (model
F-2000) at excitation wavelengths of 340 and 380 nm and emission at 510 nm. Details of the fluorometric techniques for determining
[Ca2+]i
have been described elsewhere (8, 10). EGTA (3 mM) was used in some
experiments to lower extracellular
[Ca2+]i
to 150 nM. IP3-mediated
Ca2+ release in T cells was
carried out after permeabilizing the cells with saponin (150 µg/ml),
as described earlier (15).
[Ca2+]i
were recorded after calibration of the fluorescent signals using
Ca2+ standard solutions (27).
Results were digitized and imported into a statistical analysis program
(Statistical package for Social Sciences Software Program, version 2.0;
SigmaStat, Chicago, IL) for quantitative analyses. Normalized
[Ca2+]i
responses shown in some figures were calculated in the following two
steps: 1) the lowest basal
[Ca2+]i
was subtracted from all of the
[Ca2+]i
values, and 2) the resulting
[Ca2+]i values were divided by
maximum [Ca2+]i value.
This allowed us to hold the maximum
[Ca2+]i
equal to one and then express remaining
[Ca2+]i
values as fractions of one. Integrated
[Ca2+]i
were determined by calculating the area under the
[Ca2+]i
response curve; the integrated
[Ca2+]i
values were pooled separately for control and experimental groups and
were presented as means ± SE. Unless mentioned, integrated [Ca2+]i
in T cells were calculated over the period of 300 s starting from the
time of concanavalin A (Con A) stimulation. In the present study, we
determined the effects of various Con A concentrations on T cell
[Ca2+]i
elevation and found T cell stimulation to be maximal at the 100-µg/ml
concentration. Therefore, we employed the 100-µg/ml concentration in
this series of experiments. We used 10 µM PGE2 in all
PGE2-related experiments.
The data, wherever applicable, are presented means ± SE and were
analyzed using ANOVA (Statistical package for Social Sciences Software
Program, version 2.0; SigmaStat). A P < 0.05 between the two groups was considered as statistically
significant. The experiments described here were conducted in adherence
to the National Institutes of Health Guidelines for the Care and
Use of Laboratory Animals.
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RESULTS |
[Ca2+]i
images in individual T cells before and ~150 s after their
stimulation with the mitogen (Con A) are shown in Fig.
1. In unstimulated conditions, almost all
cells appeared blue, a color corresponding to 20-60 nM
[Ca2+]i
as shown on the pseudocolor scale bar (Fig.
1A). Similarly, unstimulated T
cells incubated with PGE2 also
exhibited a color that corresponds to 20-60 nM
[Ca2+]i
(Fig. 1C). Addition of Con A caused
an increase in
[Ca2+]i
to different levels in different cells. Such
[Ca2+]i
increases ranged from 90 to 200 nM (Fig.
1B). The stimulation of cells with
Con A after PGE2 treatment failed
to cause an increase in
[Ca2+]i
(Fig. 1D). As can be seen from Fig.
2A, 85 ± 5.2% of unstimulated T cells had
[Ca2+]i
50 nM, which is likely the basal
[Ca2+]i.
After stimulation with Con A, 40 ± 8.7% of the cells maintained [Ca2+]i
50 nM, suggesting that the remaining ~60% of the basal state cells
were activated by Con A to attain
[Ca2+]i
50 nM. Con A apparently caused increases in the number of cells with
[Ca2+]i
at 100, 150, and 200 nM. PGE2 did
not have a demonstrable effect on
[Ca2+]i
distribution before stimulation of cells with Con A (Fig.
2B). In the
PGE2-treated group,
[Ca2+]i
was 50 nM in 88 ± 0.9% of the unstimulated cells and 72 ± 9% of Con A-stimulated cells, suggesting that Con A caused increases in
[Ca2+]i
in only ~16% of the
PGE2-treated cells. This level of
stimulation by Con A is apparently less than that observed in the
untreated T cells.
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Fig. 1.
Pseudocolor representation of intracellular
Ca2+ concentration
([Ca2+]i)
level in fura 2-loaded T cells.
A: T cells without concanavalin A (Con
A) stimulation. B: T cells ~150 s
after Con A stimulation. C:
PGE2-treated T cells without
stimulation. D:
PGE2-treated T cells ~150 s
after Con A stimulation. Treated T cells were incubated with 10 µM
PGE2 for ~60 min before
[Ca2+]i
measurements.
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Fig. 2.
Distribution of
[Ca2+]i
in T cells before and after stimulation with Con A. A: T cells without
PGE2 treatment.
B: T cells with
PGE2 treatment. T cells from each
of 5 rats were divided into 2 batches; cells of 1 batch were incubated
with PGE2 (see legend to Fig. 1).
Approximately 200 cells from 1 batch were first imaged for
[Ca2+]i
before they were stimulated with Con A and then were reimaged after Con
A. A similar number of cells from the batch treated with
PGE2 were also imaged before and
after Con A. Image analyses yielded numbers of cells with a given
[Ca2+]i
that ranged from 20 to 250 nM. The number of cells with a given
[Ca2+]i
was determined in the cell population from each rat before and ~150 s
after stimulation with Con A. For the percentage determination, a
scatter graph (y-axis showing
[Ca2+]i
for each of the ~200 cells, nos. 1-200, represented on the
x-axis) of
[Ca2+]i
in these cells was generated using imaging software (Metamorph; UIC,
Westchester, PA). Scatter graph was analyzed visually by counting cells
in each of the several
[Ca2+]i
ranges of 25-50 nM, 51-100 nM, 101-150 nM, 151-200
nM, and 201-250 nM and determining percentage of cells in each
concentration range (of the total ~200 cells). Percentage of cells in
the various concentration ranges was again determined after exposing
these cells to Con A. Similarly,
[Ca2+]i
were determined in the same 200 cells 150 s after Con A
stimulation, and
[Ca2+]i
values in different categories were grouped as described above. The
percentage of cells in a category was determined by calculating number
of cells in that category per total number of T cells analyzed. Percent
responsiveness in a population was determined by calculating the
difference in the responses observed before and after stimulation of T
cells with Con A. Values shown represent means ± SE from 5 rats.
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The loss of
[Ca2+]i
response to mitogen in
PGE2-treated T cells could result
from a decrease either in Ca2+
release from intracellular stores, from a decrease in
Ca2+ influx, or both. We first
determined the kinetics and relative contributions of these two
mechanisms in T cell suspensions without added
PGE2. Without the exposure of
cells to EGTA, the stimulation by Con A resulted in a rapid increase in
[Ca2+]i
followed by a slow recovery (over an ~200-s duration) that was
incomplete and then by a second slowly rising phase of the [Ca2+]i
(Fig.
3A). In
the presence of 3 mM EGTA, the kinetics and the magnitude of the
initial rise in
[Ca2+]i
were not different from those observed in the absence of EGTA. However,
the subsequent decline in
[Ca2+]i
was more rapid and was not followed by the second rise in
[Ca2+]i
(Fig. 3B). The second rise in
[Ca2+]i
in the absence of EGTA was presumably due to
Ca2+ influx (Fig.
3C). We compared the areas under the
[Ca2+]i
curves to estimate integrated
[Ca2+]i
responses (over the period of 300 s starting from time of Con A
addition to the cells) in the absence and presence of EGTA. Con A
caused an increase in integrated
[Ca2+]i
(3.51 ± 0.22 × 104
nM/s, mean ± SE from 8 different animals) in the
absence of EGTA that was significantly higher
(P < 0.05) than that obtained in the
presence of EGTA (1.07 ± 0.05 × 104 nM/s). The difference between
the two
[Ca2+]i
responses (~2.44 × 10
4 nM/s) probably
represented the magnitude of Ca2+
influx from the extracellular space in cells stimulated with Con A. The
integrated responses indicate that, during the initial 300 s of Con A
simulation of control T cells, ~40% of the total [Ca2+]i
originated from the intracellular stores and ~60% originated from
the extracellular pool. These data showed also that the Con A-mediated
initial rapid rise in
[Ca2+]i
in control T cells was primarily due to release of
Ca2+ from the intracellular stores
and that Ca2+ influx was initiated
after peak
[Ca2+]i
was achieved. This finding provided us with the rationale for examining
the effect of PGE2 on
Ca2+ influx by applying it to T
cells at the time of peak
[Ca2+]i
response to the mitogen. PGE2
addition at the peak
[Ca2+]i
(attained at ~100 s after Con A stimulation) increased the rate of
the subsequent decline in
[Ca2+]i
relative to that observed in the absence of
PGE2 (Fig.
4). Furthermore, we found that
[Ca2+]i
elevation in the presence of PGE2
returned to the basal level in ~300 s, whereas, in the presence of 3 mM EGTA, this took ~200 s. Because the rate of
[Ca2+]i
decline with PGE2 was still slower
than that which occurred in the presence of EGTA, it can be surmised
that PGE2 causes a net decrease in
cytosolic
[Ca2+]i
accumulation by decreasing Ca2+
influx.
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Fig. 3.
Representative traces from spectrophotofluorometric assessments of Con
A-induced
[Ca2+]i
in T cells in the presence and absence of 3 mM EGTA.
A:
[Ca2+]i
before and after stimulation of T cells with Con A. B: Con A-induced
[Ca2+]i
response in T cells in the presence of 3 mM EGTA.
C: composite of normalized
[Ca2+]i
responses in A and
B. Details of normalized
[Ca2+]i
are given in EXPERIMENTAL PROCEDURES.
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Fig. 4.
Representative traces from spectrophotofluorometric assessments showing
the effects of PGE2 or EGTA on the
Con A-mediated
[Ca2+]i
response in T cells. Traces are typical of results obtained from cells
of 8 different animals. Normalized
[Ca2+]i
response was calculated as described in EXPERIMENTAL
PROCEDURES.
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We also examined the effects of the second messenger of
PGE2, cAMP, by applying DBcAMP to
T cells at the peak
[Ca2+]i
response to Con A. Like PGE2,
DBcAMP augmented the rate of decline of
[Ca2+]i.
The
[Ca2+]i
decline to basal level in the presence of DBcAMP occurred over a time
period comparable to that observed with
PGE2 (~540 s after Con A). To
compare the effects of PGE2 with
that of DBcAMP on Ca2+ influx, we
integrated the area under the
[Ca2+]i
response curve from 340 s after Con A addition to the time of return of
[Ca2+]i
to near basal levels, a time interval during which the
[Ca2+]i
elevation was presumably due to influx alone (Fig.
3C). The average integrated
[Ca2+]i
response values obtained from T cells of eight different animals are
shown in Fig. 5. In the absence of
PGE2 or DBcAMP, the integrated [Ca2+]i
in T cells after their stimulation with Con A was found to be 2.15 ± 0.35 × 104 nM/s. This
[Ca2+]i
response was significantly (P < 0.01) suppressed when the cells were treated with
PGE2 or DBcAMP after Con A
stimulation.
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Fig. 5.
Effect of PGE2 (10 µM) and
dibutyryl-cAMP (DBcAMP, 1 mM) on Con A-induced T cell integrated
[Ca2+]i
response during the time interval that presumably allowed
Ca2+ influx, for the most part.
The time period selected (~340-540 s after the addition of Con
A) began at the presumed end of the release of intracellular
Ca2+ and ended at the return of
[Ca2+]i
response to near basal levels. Integrated
[Ca2+]i
were estimated as described in EXPERIMENTAL PROCEDURES.
Data (means ± SE) represent measurements in T cells from 8 different animals. * P < 0.01, Con A vs. Con A + PGE2
or Con A + DBcAMP.
** P < 0.05, Con
A + PGE2 vs. Con
A + DBcAMP by ANOVA.
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A more definitive PGE2 effect on
Ca2+ influx is indicated by data
in Fig. 6. Thapsigargin, which presumably
inhibited Ca2+ uptake into the
intracellular reservoir and caused depletion of the reservoir, allowed
for the monitoring of Ca2+ influx
after CaCl2 was added to the
extracellular compartment. Figure 6 shows a cessation of the
Ca2+ influx with the
reintroduction of additional quantities of EGTA. PGE2 addition after
CaCl2 was evidently effective in
attenuating the influx of Ca2+.
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Fig. 6.
Representative traces from spectrophotofluorometric assessments showing
the effects of PGE2 (10 µM) on
Ca2+ entry in T cells when there
was no refilling of the intracellular stores. Thapsigargin (100 nM) was
used to inhibit Ca2+-ATPase pump.
EGTA (3 mM) and CaCl2 (3 mM) were
used, respectively, to chelate and replenish
Ca2+ in the medium. Traces are
typical of T cells from 5 different animals.
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To assess the potential effect of
PGE2 on intracellular
Ca2+ release, 10 µM
PGE2 was first added to T cells
followed by the addition of 3 mM EGTA 100 s later. Con A was then added
when a stable T cell
[Ca2+]i
was established, ~100 s after EGTA. T cell
[Ca2+]i
changes after these additions are shown in Fig.
7, A and
B. In these experiments, we noticed a
higher basal
[Ca2+]i
in T cells (Fig. 7, A and
B). The
[Ca2+]i
was reduced to ~70 nM after adding 3 mM EGTA. As shown in
Fig. 7, Con A-induced Ca2+ release
in the presence of EGTA and PGE2
(0.94 ± 0.16 × 104 nM/s,
mean integrated
[Ca2+]i ± SE values obtained from 6 different animals) was not
significantly different from that observed in T cells exposed to EGTA
alone (0.95 ± 0.15 × 104
nM/s, mean integrated
[Ca2+]i ± SE values obtained from 6 different animals). In some
experiments, we used IP3 to
directly stimulate the
IP3-sensitive
Ca2+ reservoirs in T cells with or
without pretreatment with PGE2. Cells were first permeabilized with saponin (150 µg/ml) for
~40-60 min and then were stimulated with
IP3 after their exposure to PGE2. After establishing a stable
[Ca2+]i
with 3 mM EGTA, addition of 50 µM
IP3 in the absence of
PGE2 induced an elevation in
[Ca2+]i
from ~60 to ~140 nM (Fig. 7C).
The IP3-induced
Ca2+ release in the presence of
PGE2 did not appear to be
different from that in its absence (Fig.
7D). These experiments suggested that Con A stimulation of T cells ~100 s after their exposure to
PGE2 did not have a significant
effect on intracellular Ca2+
release. Furthermore, T cell release of
Ca2+ by
IP3 was also not affected when
PGE2 was added to T cells 100 s
before IP3. These results are in
contrast to our previous findings of the effect of 2 h of exposure of T
cells to PGE2 (10). In the
previous studies, we showed a suppression in the initial rise in
[Ca2]i
elevation in T cells preincubated with
PGE2 for 2 h. As we found in this
study, the initial rise is primarily due to
Ca2+ release from intracellular
stores. A suppression in the initial Ca2+ rise in T cells incubated
with PGE2 for 2 h could also
result from a decrease in Ca2+
release from intracellular stores. To elucidate the effects of long-term exposure (~2 h pretreatment) of
PGE2 on T cell intracellular Ca2+ release, we have now examined
Ca2+ release in the presence of
EGTA (Fig. 8). We found that Con A-mediated [Ca2+]i
elevation in the presence of 3 mM EGTA was significantly
(P < 0.01) suppressed in the T cells
preincubated with PGE2 (0.81 ± 0.05 × 104 nM/s, mean
integrated
[Ca2+]i ± SE values obtained from 6 different animals) compared with T
cells incubated without PGE2 (1.21 ± 0.08 × 104 nM/s, mean
integrated
[Ca2+]i ± SE values obtained from 6 different animals). These data indicated that a prolonged incubation of T cells with
PGE2 led to a decrease in both
Ca2+ influx and release from
intracellular stores.
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Fig. 7.
Representative traces from spectrophotofluorometric assessments showing
the effects of PGE2 on
Ca2+ release from intracellular
reservoir after stimulation with Con A
(A and
B) or inositol 1,4,5-trisphosphate
(IP3;
C and
D). For
IP3-mediated release, T cells were
permeabilized by incubating with saponin (150 µg/ml) for 30-45
min at room temperature. Traces are typical of results obtained from
cells of 6 different animals.
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Fig. 8.
Representative traces from spectrophotofluorometric assessments showing
effects of PGE2 on Con A-mediated
[Ca2+]i
elevation in T cells in the presence of 3 mM EGTA. T cells were
incubated with and without PGE2
(10 µM) for 2 h before
[Ca2+]i
measurements at 37°C. Traces are typical of results obtained from
cells of 6 different animals.
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DISCUSSION |
The role of PGE2 as an
immunosuppressant has been amply established (8, 18, 20, 33).
Specifically, PGE2 is known to
suppress T cell IL-2 production and proliferation (6, 7, 8, 10, 18, 20,
23, 24, 34). A number of studies have shown burn/sepsis injury-related
alterations in T cell IL-2 transcriptional regulation (6, 24, 28).
Previous studies from our laboratory have shown an impairment in T cell
early signaling events, including intracellular
Ca2+ mobilization in sepsis (8,
9). We showed also that the treatment of septic animals with the
PGE2 blocker indomethacin prevented the sepsis-related suppression in T cell
Ca2+ signaling and the
proliferative responses (8, 10). Similar changes in
Ca2+ signaling were implicated in
trauma-induced T cell functional disturbances (20). On the other hand,
Faist et al. (16) suggested a primary role of protein kinase C
(PKC) in trauma-related suppression of T cell
proliferation. The role of PKC in
PGE2-mediated T cell proliferative
disturbances was also supported by the studies of Chouaib et al. (7).
They suggested that, although PGE2
affected both Ca2+ mobilization
and PKC activation, the restitution of
Ca2+ signal partially restored T
cell proliferation, whereas PKC activation via tetradecanoylphorbol
13-acetate (TPA) completely restored the T cell response. This is
understandable because, although the activation of some PKC isoforms is
dependent on Ca2+, certain other
isoforms are independent of Ca2+.
TPA stimulation would be expected to have near-maximal stimulation of
both Ca2+-dependent and
-independent PKC, leading to an abrogation of the PGE2-mediated suppression.
Stimulation of T cells with mitogen or antigen results in a cascade of
intracellular events, including elevation in
[Ca2+]i
and PKC activation (1, 2, 4, 33). Recent studies have suggested that
the sustained elevation in
[Ca2+]i
for several hours is critical for T cell IL-2 production and subsequent
proliferation (2, 4, 21, 37).
Recent studies have shown that anti-CD3 or mitogen stimulation of T
cells induced Ca2+ signals of
diverse magnitudes in a population of T cells and that only
20-30% of the cells responded to such stimuli (19). These
findings would imply that effects of
PGE2 on T cell
Ca2+ signaling are likely mediated
through the action of PGE2 action on the 20-30% anti-CD3 or mitogen-sensitive cell population. Our previous assessments of Ca2+
signaling in T cell suspensions had also indicated variations in
responsiveness within the T cell population. In the present study,
Ca2+ imaging in individual T cells
indicated that the addition of Con A to control T cells elevated
[Ca2+]i
in ~50-60% of the cells present in the microscopic field. The difference in our finding and the earlier study indicating 20-30% responsive cells could be due to the different sources of the T cells
studied. The mitogen-responsive control rat T cell population was
comprised of ~43% cells showing a 2-fold increase in their [Ca2+]i
and 15-20% cells with a 5- to 10-fold increase. Clearly,
PGE2 suppressed
[Ca2+]i
in all responsive T cells, regardless of the level of their responsiveness to the mitogen. Based on the color distribution in
unstimulated T cells, there seems to be a tendency of decrease in the
basal
[Ca2+]i
in PGE2-treated T cells (Fig.
1C) compared with unstimulated T
cells incubated in the absence of
PGE2 (Fig.
1A). However, this decrease was
not demonstrable when the data were pooled from five different animals
(Fig. 2).
Previous studies suggested that the
PGE2-related decrease in T cell
Ca2+ signaling could be due to a
PGE2-mediated inhibition of
PIP2 hydrolysis and the subsequent
IP3 production (3, 7, 17, 21-23). These studies implied that the decrease in
IP3 production could lead to a
decreased release of Ca2+ from the
intracellular reservoir. However, Gouy et al. (17) found that, despite
a decrease in IP3 production
occurring after treatment of T cells with cholera toxin, there was no
change in Ca2+ release from the
intracellular reservoir. Our present study demonstrated a decrease in
Ca2+ release from intracellular
stores when T cells were preincubated with
PGE2 for 2 h, although the
treatment of T cells with PGE2 immediately before their stimulation with Con A or at peak
[Ca2+]i
response to Con A failed to affect the capability of intracellular stores to release Ca2+ or the
sensitivity of the release mechanism to
IP3. These findings suggest that,
although prolonged exposure of T cells to
PGE2 (2 h) before cross-linking of
the TCR with Con A could attenuate Con A-mediated formation of
IP3, such
IP3 generation may not be compromised immediately after PGE2
application to T cells. We speculate that the trigger for
Ca2+ release from intracellular
stores may be affected only after the prolonged
PGE2 exposure.
Previous studies have shown that, although
Ca2+ influx is important in the
maintenance of the sustained elevation of T cell [Ca2+]i
(2, 5, 14, 21, 37), all of the
Ca2+ entering the cell may not
contribute to the
[Ca2+]i
elevation. Some of the Ca2+ are
presumably either extruded via a
Ca2+ efflux mechanism or pumped
into the intracellular Ca2+ stores
(4, 14, 29). An alteration in any of these mechanisms could also affect
the sustained Ca2+ elevation. As
pointed out in RESULTS, the influx of
Ca2+ was observed (Fig. 6) in T
cell depleted of the intracellular Ca2+ store. The influx of
Ca2+ in store-depleted cells
represents a store-dependent influx pathway referred to as the
"capacitive Ca2+ entry" (31,
32). A number of recent studies suggested that capacitive
Ca2+ entry in various cell
systems, including the T cells, is activated by the depletion of the
Ca2+ store and is terminated by
subsequent refilling (13, 29, 30, 38). We evaluated the effects of
PGE2 on
Ca2+ entry in T cells after their
exposure to thapsigargin in the presence of 3 mM EGTA. In the presence
of EGTA, thapsigargin allowed for the depletion of the
Ca2+ stores and prevented their
refilling. The results in Fig. 6 showing the elevation in
[Ca2+]i
after restitution of Ca2+ in the
extracellular medium suggest capacitive
Ca2+ entry in rat T cells. These
studies are consistent with earlier observations in human transformed
Jurkat T cells and other cell systems (13, 31). The elevation in T cell
[Ca2+]i
in the presence of thapsigargin was presumably due to entry from
extracellular medium, as reintroduction of EGTA led to return of
[Ca2+]i
to basal levels. Similar to EGTA, addition of
PGE2 also produced a marked
suppression in
[Ca2+]i
elevation. These results supported the hypothesis that the PGE2-mediated decrease in
sustained elevation could also result from an attenuation in a
capacitive Ca2+
entry. The decrease in
[Ca2+]i
elevation due to a decrease in
Ca2+ influx and its release from
intracellular stores is likely a major contributor to
PGE2-mediated suppression of T
cell responses.
| |
ACKNOWLEDGEMENTS |
Technical assistance by Dr. Z. Ahmed and L. Amato is acknowledged.
| |
FOOTNOTES |
This study was supported by National Institute of General Medical
Sciences Grants RO1GM-53235 and RO1GM-56865.
The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement"
in accordance with 18 U.S.C. §1734 solely to indicate this fact.
Address for reprint requests and other correspondence: M. M. Sayeed,
Burn and Shock Trauma Institute, Loyola Univ. Chicago Medical Center,
2160 South First Ave., Maywood, IL 60153 (E-mail:
msayeed{at}luc.edu).
Received 2 March 1999; accepted in final form 26 July 1999.
| |
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