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IMMUNOBIOLOGY
From the Department of Pathology, Harvard Medical
School, and The Center for Blood Research, Boston, MA; the Department
of Medicine I, University Hospital Carl Gustav Carus, Dresden
University of Technology; and the Max-Planck-Institute for Infection
Biology, Berlin, Germany.
Transcription factors of the nuclear factor of activated T cells
(NFAT) family are thought to regulate the expression of a variety of
inducible genes such as interleukin-2 (IL-2), IL-4, and tumor necrosis
factor- In response to antigen stimulation, cells of the
immune system initiate the expression of activation-induced genes
through the coordinate action of transcription factors at gene
regulatory elements. The nuclear factor of activated T cells (NFAT),
originally identified as a nuclear complex binding to the
antigen-response element of the IL-2 gene,1 has been
implicated in the regulation of various inducible genes, particularly
those encoding cytokines and cell surface receptors.2
Sequence inspection, in vitro binding assays, and overexpression
studies have identified potential binding sites for NFAT in the
promoters and enhancers of numerous genes, including those encoding
interleukin-2 (IL-2), IL-3, IL-4, IL-5, tumor necrosis factor To date, 4 calcium-regulated members of the NFAT family (NFAT1-4; also
known as NFATc1-4 and hereafter abbreviated NFAT), with distinct but
overlapping tissue distributions, have been identified.8-15 A fifth protein,
NFAT5/TonEBP,16,17 is regulated by osmotic shock. NFAT3 is
expressed predominantly outside the immune system, whereas NFAT1
(NFATp, NFATc2), NFAT2 (NFATc, NFATc1), and NFAT4 (NFATx, NFATc3) can
be found in immune cells including T cells, B cells, natural killer
(NK) cells, macrophages, and mast cells.2,10,18-21
Although NFAT proteins are expressed in multiple cell types, their
regulation has been extensively studied in T and B cells, where they
are present as phosphoproteins in the cytoplasm of resting cells. After
cell stimulation, 4 consecutive steps lead to the activation of NFAT:
dephosphorylation by the calcium-dependent phosphatase calcineurin, a
process inhibited by the immunosuppressive drugs cyclosporin A and
FK50622-26; translocation into the
nucleus18,23,27; binding to specific DNA elements in
the regulatory regions of target genes, which occurs in physical or
functional cooperation with other transcription factors including AP-1
(Fos/Jun), c-Maf (Maf), and GATA-family
proteins2,4,22,28-30; and interaction with known or
putative coactivator proteins such as p300, CBP, and
NIP-45.31-33
After antigen stimulation, CD4+ T cells differentiate into
at least 2 types of effector cells that differ as to the pattern of
cytokines they produce on restimulation.34-36 Th1 cells
are defined by the production of interferon- We and others42-44,53 have previously shown that T cells
isolated from NFAT1-deficient mice have a strong bias to differentiate into Th2 cells. Detailed analysis traced this phenotype to the fact
that NFAT1 To eliminate the skewing effects caused by IL-4 overexpression in
NFAT1 Mice
Cell culture conditions and reagents
For primary stimulation, purified CD4+ T cells (1 × 106/mL) were stimulated in vitro for the indicated time points with 1 µg/mL plate-bound anti-CD3 (2C11; Pharmingen, San Diego, CA) or the combination of 10 ng/mL IL-12 (courtesy of M. O'Donnell, Genetics Institute, Cambridge, MA) and 50 ng/mL IL-18 (gift of M. Su, Vertex Pharmaceuticals, Cambridge, MA). In vitro differentiation assays were performed as described.44 Briefly, purified CD4+ T cells (1 × 106/mL) were stimulated with 1 µg/mL plate-bound anti-CD3 alone (default conditions) or in the presence of 5 ng/mL IL-12 or the indicated amounts of IL-4 (IL-4 was added as supernatant from the cell line I3L6 transfected with a constitutively expressed murine IL-4 cDNA55). All cultures were supplemented with 20 U/mL IL-2 (Collaborative Biomedical Products, Bedford, MA) after 24 hours, and fresh media (30% of the initial volume) was added after 48 hours of stimulation. After 4 days, cells were extensively washed, rested for 24 to 48 hours in IL-2 (20 U/mL), counted, and restimulated at 1 × 106 cells/mL with 1 µg/mL plate-bound anti-CD3 for the indicated time points. For mixing experiments, NFAT1+/+ IL-4 Transfections Plasmid DNA (0.75 µg/106 cells) was introduced in Cl.7W2 cells58 by electroporation in serum-free medium in 0.4-cm cuvettes with settings of 250 V and 950 µF, using a Bio-Rad Gene Pulser II (Hercules, CA). The day after transfection, cells were stimulated for intracellular cytokine staining as indicated.Enzyme-linked immunosorbent assay and intracellular cytokine staining Culture supernatants of cells activated as described above were collected at 24 hours (secondary stimulation) or 48 hours (primary stimulation), and cytokine levels for IFN- , IL-2, and IL-5 were
analyzed by enzyme-linked immunosorbent assay (ELISA) using standard
protocols and monoclonal antibodies specific for murine (m) IFN-,
mIL-2, and mIL-5 (courtesy of A. Clausell, Pharmingen). Calculated
values are expressed as mean ± SEM.
For intracellular cytokine staining, differentiated T cells or Cl.7W2
cells were stimulated with 20 nM phorbol 12-myristate 13-acetate
(PMA) and 1 µM ionomycin for 4 to 5 hours, the last 2 hours
in the presence of 10 µg/mL Brefeldin A (Sigma). After harvest, cells
were washed with cold phosphate-buffered saline (PBS), fixed for 10 minutes in 4% paraformaldehyde, washed twice with PBS, and
permeabilized with PBS/FCS containing 0.5% saponin (Sigma). Staining
was performed for 30 minutes at room temperature with allophycocyanin-
or phycoerythrin-conjugated control immunoglobulin and anti-mIFN- RNase protection assay and Northern blot analysis At the indicated time points after stimulation, cells were harvested and total cellular RNA was immediately extracted (Ultraspec, Houston, TX). Cytokine mRNA levels were analyzed by RNase protection assay using the RiboQuant multiprobe kit (Pharmingen) following the instructions of the manufacturer. Briefly, equal amounts of target RNA (1-5 µg) were hybridized overnight to a [32P]-labeled RNA probe that had been synthesized in vitro from a multicytokine template set, after which free probe and other single-stranded RNA were digested with RNases. Protected fragments were purified and resolved on a 6% denaturing polyacrylamide gel and visualized by autoradiography. Cytokine transcripts were identified by the lengths of the respective fragments. RNA loading was estimated by measuring intensities of protected fragments encoding 2 housekeeping genes, L32 and GAPDH, included in the multitemplate set as internal controls.For Northern blot analysis, total RNA was separated by gel electrophoresis (10 µg/lane) and transferred to a nylon membrane (Nytran; Schleicher & Schuell, Keene, NH). cDNA fragments for Northern hybridization were purified from plasmids containing the full-length murine c-Maf30 and human GATA-359 cDNAs, respectively. Infections with Leishmania major L major LRC-L137 clone V121 promastigotes60 were cultured in semidefined medium 7961 supplemented with 10% FCS (Seromed, Berlin, Germany) to stationary phase at 26°C. The cells were harvested and washed twice with PBS and finally resuspended in PBS at 108 parasites/mL. Thirty microliters of this suspension was injected into the left hind footpad. Footpad thickness was recorded at the indicated times using a caliper. The difference to the uninfected foot was calculated and plotted as the mean ± SD.Parasite burden in draining lymph nodes was estimated by limiting-dilution analysis. Single-cell suspensions of lymph node cells were serially diluted by a factor of 3.18 in 4 replicates in semidefined medium 79. Parasite growth was recorded microscopically after 4 to 6 days of culture. Total number of parasites per lymph node was calculated from the highest dilution at which a minimum of 1 of 4 replicates still contained parasites and the total number of lymph node cells in suspension.
All the experiments described in this article were performed using
IL-4-deficient T cells that either expressed or lacked the
transcription factor NFAT1. For simplicity, therefore, the cells are
occasionally referred to as NFAT1 NFAT1 regulates IFN-  / and NFAT1/ IL-4/
spleen and lymph node cells and differentiated them in vitro with
plate-bound anti-CD3, in the absence of added cytokines or antibodies
(default conditions). Four days after stimulation, cells were washed,
rested, and restimulated with plate-bound anti-CD3, after which levels
of cytokine transcripts were quantified by RNase protection assay
(Figure 1A). Under these conditions, both NFAT1+/+ IL-4/ and NFAT1/
IL-4/ T cells expressed barely detectable levels of
mRNAs encoding the Th2 cytokines IL-5 and IL-13 and, as expected, no
mRNA encoding IL-4 (Figure 1A, left panel). This result confirmed our
earlier conclusion that Th2 differentiation in NFAT1/
cells was completely dependent on IL-4 because it was inhibited by
inclusion of a neutralizing anti-IL-4 antibody.44,53 In the same experiment, NFAT1/ IL-4/ T
cells expressed considerably lower levels of mRNA encoding GM-CSF and
the Th1 cytokine IFN- than NFAT1+/+
IL-4/ T cells (Figure 1A). In contrast, there was no
consistent difference in the expression of IL-2, FasL, and TNF-
between NFAT1/ IL-4/ and
NFAT1+/+ IL-4/ T cells (Figure 1A-B, right
panel). Analysis of supernatants of restimulated cells by ELISA
confirmed that IFN- production by NFAT1/
IL-4/ T cells was profoundly compromised (Figure 1B,
left panel). These experiments suggested that NFAT1 acted independently
of IL-4 to regulate IFN- and possibly GM-CSF expression during
T-cell differentiation.
As shown previously, Th2 skewing of NFAT1
NFAT1 regulates IFN- -producing cells during T-cell differentiation. To examine the involvement of
soluble or membrane-bound factors that might influence IFN- production, we performed mixing experiments in which
NFAT1/ IL-4/ and NFAT1+/+
IL-4/ T cells were differentiated either alone or
together. To distinguish the 2 types of T cells in the mixed
populations, we labeled one of the populations with the fluorescent dye
CFSE.57 After differentiation, IFN- production by
NFAT1/ IL-4/ and NFAT1+/+
IL-4/ T cells was independently quantified, either by
restimulation followed by intracellular cytokine staining (Figure
3A) or by separating differentiated cells
by cell sorting, restimulating the separated populations, and measuring
IFN- by ELISA assays of cell supernatants (Figure 3B). As shown in
Figure 3, NFAT1/ IL-4/ T cells
consistently produced less IFN- than NFAT1+/+
IL-4/ T cells, regardless of whether they were labeled
with CFSE and whether they were cultured alone or together with the
other cell type. This result suggested that NFAT1 promotes IFN-
production by differentiated T cells through a cell-intrinsic mechanism
rather than indirectly by inducing soluble or membrane-bound
factors.
We asked whether reduced IFN-
NFAT1 is required for optimal IFN- production by effector T
cells.62 The experiments reported above involved purified
CD4+ T cells and thus did not reflect IL-12-dependent
mechanisms. We therefore asked whether the inclusion of IL-12 during
differentiation would rescue high levels of IFN- production in
NFAT1/ IL-4/ relative to
NFAT1+/+ IL-4/ T cells. In the same
experiment, we asked whether the IFN- defect of these cells was
limited to a restricted time window or was maintained through several
rounds of differentiation involving repeated restimulations. To avoid
the potentially confounding effects of CD4+ memory or NK1.1
T cells, we used naive T-cell populations (CD4+
Mel-14hi) of NFAT1/ IL-4/
and NFAT1+/+ IL-4/ cells. Cells were
cultured in the absence or presence of IL-12 for 2 consecutive
rounds of differentiation involving a total of 3 stimulations the
primary stimulation (depicted as number 1 in Figure
5), the secondary stimulation (number 2)
occurring after the first round of differentiation, and the tertiary
stimulation (number 3) occurring after the second round of
differentiation. After each stimulation, supernatants (Figure 5) and
total RNA (data not shown) were analyzed for IFN-
expression.
Strikingly, a marked reduction in IFN- Decreased resistance of NFAT1 is critical for resistance to
infections with intracellular pathogens, such as L major. To
test whether the reduced IFN- production by NFAT1/
IL-4/ T cells had biologically relevant consequences in
vivo, we infected NFAT1/ IL-4/ and
NFAT1+/+ IL-4/ mice with L major
in one hind footpad. As expected from both their IL-4 null and their
C57BL/6 and 129/SvJ genetic backgrounds,63 both mouse
strains were considerably resistant to the infection and eventually
controlled the disease (Figure 6A).
However, compared to footpads of NFAT1+/+
IL-4/ mice, footpads of NFAT1/
IL-4/ mice showed a slight but significant increase in
size during the course of the infection (Figure 6A). This was
paralleled by an approximately 10-fold increase in the number of
parasites (Figure 6B; note logarithmic scale), and a 2-fold increase in
the number of lymphocytes (data not shown), in the draining lymph nodes
of NFAT1/ animals 11 weeks after infection. These
results suggested that resistance to infection with L major
was reduced in NFAT1/ IL-4/ mice
compared to IL-4/ mice and is consistent with reduced
IFN- production by NFAT1/ IL-4/
relative to IL-4/ CD4+ T cells.
NFAT1 is required for the acute phase of IFN- gene expression in naive T cells. To test this
hypothesis further, we asked whether freshly isolated, undifferentiated NFAT1/ IL-4/ T cells would show
impaired IFN- production in response to stimuli that do not involve
activation of NFAT proteins (Figure 7A).
The stimuli chosen were IL-12 and IL-18, cytokines that activate STAT and NF B proteins, respectively, but are not known to activate NFAT.35,36,64 As shown in Figure 7A,
NFAT1/ IL-4/ T cells stimulated by
anti-CD3 for 48 hours produced substantially lower levels of IFN-
than NFAT1+/+ IL-4/ T cells. In contrast,
IFN- production in response to combined stimulation with IL-12 and
IL-18 was not impaired but was slightly enhanced in
NFAT1/ IL-4/ relative to
NFAT1+/+ IL-4/ T cells. Thus, NFAT1 appears
to be required for acute expression of the IFN- gene in T cells
through a specific CD3-mediated pathway, whereas an alternative,
IL-12- and IL-18-dependent pathway remains unaffected.
To further determine the role of NFAT in the acute phase of IFN-
In this study, we show that T cells lacking NFAT1 display a
substantial, cell-intrinsic defect in IFN- NFAT1 regulates acute transcription of the IFN- gene
transcription is complex. During Th1 differentiation, T-cell receptor-
and IL-12/STAT4-dependent signaling pathways are highly interconnected,
such that the final levels of differentiated, IFN- producing Th1
cells reflect a balance between permissive factors such as STAT4, JNK2,
and T-bet38,40,48,52 versus repressive factors such as
STAT6, GATA-3, and Maf.50,51,70 In contrast, the acute
transcriptional phase is less complex: differentiated Th1 cells produce
IFN- in response to activation through at least 2 independent
signaling pathways involving the T-cell receptor and the IL-12 and
IL-18 receptors, respectively.36,64,71,72 As discussed in
the following sections, our results implicate a role for NFAT1 in the
acute phase of IFN- gene transcription.
As a transcription factor activated by T-cell-receptor stimulation,
NFAT1 is likely to contribute to the T-cell-receptor pathway, but not
the STAT4-IL-12/NF Our results do not rule out that NFAT1 also regulates IFN- Potential NFAT-dependent regulatory elements in the
IFN- gene
transcription have been extensively studied but not yet definitively identified. Analysis of the human IFN- promoter identified NFAT sites at  280 and 160 relative to the transcription start
site.66-69 The 280 NFAT site and a previously identified
intronic site may bind both NFAT and Rel, whereas the 160 site has
the characteristics of a composite NFAT-AP-1 site.68,69 In
chromatin immunoprecipitation assays, which measure the ability of a
transcription factor to bind a regulatory element in intact cells in
vivo, the IFN- promoter is clearly capable of binding
NFAT.83 However in transient reporter assays, mutation of
either of the 2 NFAT sites only marginally reduced (approximately
2-fold) the overall inducibility of the IFN- promoter, and mutation
of both sites had only a small additional effect.66,68,69
Deletion or mutation of the 280 NFAT site considerably diminished,
but did not abolish, calcineurin sensitivity of the IFN-
promoter.66,68 Together these results indicate that
although NFAT binds strongly and selectively to the proximal IFN-
promoter region in vivo, the activity of the isolated promoter is only
weakly dependent on NFAT in transient reporter assays.
The most proximal region of the IFN- In transgenic mouse models, neither the proximal nor the distal
elements fully recapitulates the behavior of the endogenous IFN- NFAT1 may act coordinately to promote Th1 differentiation and suppress Th2 differentiation The role of NFAT1 in T-helper cell differentiation has been analyzed in several in vivo models using NFAT1 knockout mice. Targeted disruption of the NFAT1 gene in mice results in a Th2 bias,43,44,53 though this is fairly mild and poorly apparent in 1 of 3 mouse strains tested.82 The mechanism of this Th2 bias remains to be understood, but it is IL-4 dependent (Kiani et al,44 Viola et al,53 and this study), and we have postulated that it might reflect the absence of a NFAT1-regulated negative feedback loop that normally terminates the antigen-induced expression of IL-4.44 The impressive allergic phenotype of mice lacking both NFAT1 and NFAT4 suggests that these 2 NFAT proteins act in concert to down-regulate Th2 responses in vivo.45In the present study, we have identified a second role for
NFAT1
We thank A. Abbas, F. Alt, L. Glimcher, K. Murphy, and S. Orkin for plasmids and other reagents; S. Agarwal and J. Aramburu for helpful suggestions; F. Macian for help with densitometry; R. Grewal for technical assistance; and T. Bernickel for animal husbandry.
Submitted June 28, 2000; accepted April 20, 2001.
Supported by National Institutes of Health grants R01 CA-42471 and P01 AI-35297 (A.R.) and by Deutsche Forschungsgemeinschaft grants KI 605/1-1 (A.K.), KI 605/2-1 (A.K., G.E.), and AE 16/1-3 (T.A.).
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
Reprints: Anjana Rao, Department of Pathology, Harvard Medical School, The Center for Blood Research, 200 Longwood Ave, Boston, MA 02115; e-mail: arao{at}cbr.med.harvard.edu.
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| Copyright © 2001 by American Society of Hematology Online ISSN: 1528-0020 | |||||||||
gene expression by nuclear
factor of activated T cells
Top
Abstract
Introduction
) and NFAT1+/+
IL-4
) cells. CD4+ T cells from
NFAT1+/+ IL-4
