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J. Biol. Chem., Vol. 275, Issue 31, 23981-23985, August 4, 2000
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,,,
,,, and**
From Berlex Biosciences, Richmond,
California 94804, the § Cleveland Clinic Foundation,
Cleveland, Ohio, 44195, the ¶ University of Illinois, Chicago,
Illinois 60605, and the University Health Network & University
of Toronto, Toronto, Ontario M5S 3E2, Canada
Received for publication, March 24, 2000, and in revised form, May 19, 2000
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ABSTRACT |
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 TOP
 ABSTRACT
 INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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A human cell line (U5A) lacking the type I
interferon (IFN) receptor chain 2 (IFNAR2c) was used to determine the
role of the IFNAR2c cytoplasmic domain in regulating
IFN-dependent STAT activation, interferon-stimulated gene
factor 3 (ISGF3) and c-sis-inducible factor (SIF) complex
formation, gene expression, and antiproliferative effects. A panel of
U5A cells expressing truncation mutants of IFNAR2c on their cell
surface were generated for study. Janus kinase (JAK) activation was
detected in all mutant cell lines; however, STAT1 and STAT2 activation
was observed only in U5A cells expressing full-length IFNAR2c and
IFNAR2c truncated at residue 462 (R2.462). IFNAR2c mutants truncated at
residues 417 (R2.417) and 346 (R2.346) or IFNAR2c mutant lacking
tyrosine residues in its cytoplasmic domain (R2.Y-F) render the
receptor inactive. A similar pattern was observed for IFN-inducible
STAT activation, STAT complex formation, and STAT-DNA binding.
Consistent with these data, IFN-inducible gene expression was ablated
in U5A, R2.Y-F, R2.417, and R2.346 cell lines. The implications are
that tyrosine phosphorylation and the 462-417 region of IFNAR2c are independently obligatory for receptor activation. In addition, the
distal 53 amino acids of the intracellular domain of IFNAR2c are not
required for IFN-receptor mediated STAT activation, ISFG3 or SIF
complex formation, induction of gene expression, and inhibition of
thymidine incorporation. These data demonstrate for the first time that
both tyrosine phosphorylation and a specific domain of IFNAR2c are
required in human cells for IFN-dependent coupling of JAK
activation to STAT phosphorylation, gene induction, and antiproliferative effects. In addition, human and murine cells appear
to require different regions of the cytoplasmic domain of IFNAR2c for
regulation of IFN responses.
Type I interferons
(IFNs),1 IFNs A proposed STAT2 binding site on IFNAR1 has been suggested which
includes two phosphorylated tyrosines, Tyr466 and
Tyr481, in which an SH2 domain within STAT2 mediates the
binding of STAT2 to these sites. For one of these sites, critical
residues include not only Tyr466 but also valine +1 and
serine+5 carboxyl-terminal to tyrosine 466 (4). STAT binding sites on
IFNAR2c have also been proposed from in vitro results using
glutathione S-transferase-IFNAR2244-462
"pull-down" experiments, where both STAT1 and STAT2 have been shown to pre-associate with IFNAR2c, in a manner
independent of receptor phosphorylation and dimerization (5). This
pre-association entails the binding of STAT2 in the absence of STAT1.
More recent studies, using mouse L929 cells, have mapped this
constitutive binding site for STAT2 to amino acids 404-462 of IFNAR2c
(6). In addition to this constitutive site on IFNAR2c, tyrosine
phosphorylation of the proximal tyrosines (tyrosines 269, 306, 316, 318, and 336) of IFNAR2c is required, however, it is insufficient by
itself, for efficient STAT2 activation (6). Therefore, stimulation of
mouse cells expressing human IFNAR2c containing only the proximal tyrosines of IFNAR2c or the constitutive docking site with human IFN Cell Lines and Reagents--
All cell lines were purchased from
American Type Tissue Culture (ATCC) and grown at 37 °C in 5%
CO2. HT1080 or U5A cells (provided by Drs. Ian Kerr and
George Stark) were grown in Dulbecco's modified Eagle's medium (Life
Technologies, Inc.) containing 10% (v/v) bovine calf serum,
L-glutamine, and 5% penicillin and streptomycin (Life
Technologies, Inc.). U5A cells were obtained as described previously
(8). Human IFN Selection of U5A Cell Lines Stably Expressing IFNAR2c Truncation
Mutants--
U5A cells (1 × 106 cells/well) were
transfected with the corresponding plasmid using Superfectin (11).
Plasmids containing a neomycin selection marker, IFNAR2c truncations,
and the full intracellular tyrosine to phenylalanine substitutions were
constructed as described previously (6, 12). Multiple stable cell lines for each IFNAR2c mutant were selected in media containing G-418 (1.0 mg/ml). After selection, individual clones were picked and expanded; an
integration of each IFNAR2c mutant DNA was determined by polymerase
chain reaction using primer sets spanning introns. Positive clones were
further expanded and tested for their ability to bind type I IFN.
Immunoprecipitation and Immunoblotting--
Cell lines
expressing IFNAR2c truncation mutants (1 × 107 cells)
were solubilized in lysis buffer (20 mM Tris-HCl, pH 7.5, containing 1% Nonidet P-40 (v/v), 150 mM sodium chloride,
1 mM EDTA, 2.5% glycerol (v/v), 1.0 mM sodium
fluoride, 1.0 mM sodium orthovanadate, 1.0 mM
phenylmethysulfonyl fluoride, 0.5 µg/ml leupeptin, and 5.0 µg/ml
trypsin inhibitor) for 30 min at 4 °C and insoluble material removed
by centrifugation. For immunoprecipitation, the indicated antibodies
were added to each sample, incubated overnight, mixed with Protein
G-agarose (Roche Molecular Biochemicals), and resolved by
SDS-PAGE (10% Novex gels). Proteins were transferred to polyvinylidene
difluoride filters (Pro-Blot) and incubated in blocking buffer (20 mM Tris-HCl, pH 7.5, containing 0.1% Tween 20 (v/v), 150 mM sodium chloride, 1 mM EDTA, 1.0 mM sodium fluoride, 1.0 mM sodium
orthovanadate, 1.0 mM phenylmethysulfonyl fluoride, 0.5 µg/ml leupeptin, and 5.0 µg/ml trypsin inhibitor) overnight at
4 °C, incubated with the appropriate antibody and washed in blocking buffer. Following washing, the membrane was incubated with a specific second antibody (1:1000 dilution) coupled to
horseradish peroxidase for 1 h, washed three times in blocking
buffer, and developed using a chemiluminescent detection method
(Pierce). To reprobe immunoblots, membranes were incubated overnight in 0.01 M sodium citrate, pH 3.0, washed in blocking buffer,
and reprobed with the appropriate antibody.
Ligand Binding Assay--
A phosphorylated form of IFN Electrophoretic Mobility Shift Assay (EMSA)--
Gel shift
assays were performed using 32P-labeled double-stranded
oligonucleotides representing the human 2-5A oligoadenylate synthetase
IFN-sensitive response element and the m67SIE element present in the
c-fos promoter. Cell were stimulated with IFN TaqMan® and RNase Protection Assay--
Cells were
stimulated with human IFN Thymidine Incorporation Assay--
Cells were seeded (2 × 104 cells/well) in a 24-well cell culture plate and
incubated overnight in either IFN U5A is a human lung fibrosarcoma cell line that cells lacks
IFNAR2c but expresses IFNAR1. Sensitivity to type I IFNs can be restored in U5A cells upon transfection with a plasmid encoding full-length IFNAR2c (7). Therefore, U5A cells provide a human cell line
in which mutant forms of IFNAR2c can be used to determine the role of
this receptor chain in type I IFN signaling in a human cell background.
Using this approach, intracellular truncation mutants of IFNAR2c were
stably expressed in U5A cells and multiple cell lines of each clone
were analyzed with similar results. Initially, integration of cDNA
encoding IFNAR2c mutants was demonstrated in transfected U5A cells by
polymerase chain reaction (data not shown). For clones of interest,
receptor number and binding affinities were then directly determined
(Table I). High affinity binding of type
I IFNs to the receptor requires both IFNAR1 and IFNAR2c (17-19). In
this study, all cell lines examined, except U5A, bound
IFN
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
, 
, and
are required for the induction of antiviral responses in a
variety of animal species (1). Type I IFNs also elicit important
antiproliferative effects in a number of cell lines and play a major
role in mediating immunomodulatory activity (2). Cellular responses to
type I IFNs require the interaction of type I IFNs with their cognate
receptor, which is composed of two receptor subunits, IFNAR1 and
IFNAR2c (also designated and L, respectively). Once
activated, the type I IFN receptor initiates signaling events, which
culminate in the induction of a broad spectrum of IFN-responsive genes
(2, 3). One of the major signaling events coupled to receptor
stimulation is the activation of signal transducers and activators of
transcription (STATs). IFN-activated STAT transcription complexes
include heterodimers of STAT1 and STAT2 along with a DNA-binding
protein of 48 kDa present in the cell cytoplasm (3). This
IFN-stimulated gene factor 3 (ISGF3) binds to IFN-sensitive response
elements present in the promoter regions of IFN-inducible genes and
initiates gene expression (2, 3). The mechanism by which activation of the type I IFN receptor leads to STAT activation and gene expression is
unclear. It is known that early stages of signaling require IFN-induced
receptor heterodimerization of both receptor chains (2, 3). However,
the mechanism by which STATs and other regulatory proteins interact
with the human type I IFN receptor is unclear, despite some emerging
evidence of receptor interactive domains.
2 results in STAT tyrosine phosphorylation, ISGF3 formation, but
no antiviral response. Thus, in this case, efficient STAT2 activation
requires both constitutive and
phosphotyrosine-dependent binding sites on the receptor. To
further define the role of IFNAR2c in IFN signaling, we have chosen to
express mutated forms of IFNAR2c having specific modifications in its
intracellular domain, in a human cell line, U5A, which lacks IFNAR2c
(7). In this way, one can directly measure the effects of
such mutants on a variety of IFN-inducible responses, in a human
cell that contains complementary Janus kinases and STAT proteins in a
background devoid of heterologous receptor chains.
MATERIALS AND METHODS
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
1b (specific activity = 2.5 × 107 units/mg) was produced as described previously (9) and
IFN2 (specific activity = 3.0 × 108 units/mg)
was purchased from Pepro Tech Inc. IFNAR1 and IFNAR2c antiserum were
prepared as described previously (10). STAT1, STAT2, TYK2, JAK1, and
anti-phosphotyrosine antibodies (Tyr(P)) were purchased from
Transduction Laboratories or Santa Cruz Biotechnology. For detection of
activated JAK1, a specific antibody that recognizes an amino acid
sequence within JAK1 containing the activation-dependent phosphorylated tyrosines 1022 and 1023 (OPA1-03051, Affinity
BioReagents) was used.
2 was
used, and ligand binding assays were performed as described previously
(10). Ligands were phosphorylated (specific activities of 60-62
µCi/µg) as described previously (10). Binding data were analyzed
according to Scatchard (13). Nonspecific binding was determined in the
presence of a 100-fold excess of unlabeled IFN.
2 (1000 units/106 cells) or IFN1b (1000 units/106
cells) for 15 min, and cell pellets collected and processed for EMSA as
described previously (14). Reaction mixtures were separated by
electrophoresis through a 6% polyacrylamide gel and analyzed by
autoradiography (14).
2 (1000 units/106 cells),
IFN1b (1000 units/106 cells), or IFN
(1000 units/106 cells) for 17 h; whole cell pellets
collected and processed for TaqMan® analysis as described
previously (15). For RNase protection assays of gene expression, cells
were stimulated and harvested as described previously (16).
1b (1000 units/ml) or IFN2 (1000 units/ml). At time 0, complete medium containing [3H]thymidine
([methyl-3H]thymidine, specific activity = 40-60 Ci/mmol; Amersham Pharmacia Biotech) was added and
cells harvested at 4, 8, and 12 h. At each time point, cells were
washed with phosphate-buffered saline followed by, 10% trichloroacetic
acid and 100% ethanol. Prior to determining incorporation of
radioactivity, cells were solubilized in 1 M potassium
hydroxide and mixed with Ecolume scintillation fluid.
RESULTS
TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
2 with high affinity (200-500 pM) (Table I). All cell lines reported here expressed mutant IFNAR2c receptor chains at
levels equal to or greater than HT1080 cells, demonstrating that truncations or replacement of all tyrosine residues within the
cytoplasmic domain of IFNAR2c, do not affect ligand binding.
Receptor number and binding affinity
IFN-induced receptor dimerization likely leads to conformationally distinct receptor complexes, dependent on the type I IFN subtype (10, 20). Such IFN-inducible activation of IFNAR1 and IFNAR2 is independent of the phosphorylation state of the receptor subunits (21). Therefore, type I IFN receptor-binding interactions appear to be directly dependent on unique interactions of type I IFNs with the two receptor chains (22). It is assumed that IFN-induced receptor assembly leads to the specific activation of the Janus kinases, TYK2 and JAK1, and the subsequent phosphorylation of both receptor chains. The assembly of both receptor chains initiates activation of these kinases in an IFN-dependent manner.
Earlier work has demonstrated a specific association between IFNAR1 and
TYK2 and IFNAR2c and JAK1 (18, 23-26). Accordingly, to confirm that
the various truncations or mutations to IFNAR2 had no effect on
TYK2-IFNAR1 function, we examined the extent of IFN-inducible TYK2
activation in transfectants expressing variant IFNAR2c
constructs. Our data indicate that IFNAR1 function, at least in the
context of IFN-inducible TYK2 activation, is unaffected in
transfectants expressing the mutant IFNAR2c constructs, but IFNAR1-associated TYK2 activation is ablated in the U5A cells (Fig.
1A). Similarly, JAK1
activation was also observed in all mutant cell lines expressing
IFNAR2c mutants. However, JAK1 activation was not observed in
IFN-stimulated U5A cells (Fig. 1B). Therefore, Janus kinase
activation (TYK2 and JAK1) is dependent on receptor dimerization, and does not require the intracellular region distal to residue 346 in IFNAR2c or tyrosine phosphorylation of IFNAR2c.
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In order to determine the contribution of distinct regions of the
intracellular portion of IFNAR2c to STAT recruitment and activation, we
examined IFN-inducible STAT1 and STAT2 activation in each of the
transfectants expressing mutant IFNAR2c. U5A cells expressing IFNAR2c
truncation mutants were stimulated for 15 min with either IFN2 (1000 units/106 cells) or IFN1b (1000 units/106
cells) and the level of STAT1 or STAT2 activation determined by
measuring the extent of STAT1 or STAT2 tyrosine phosphorylation. In
contrast to U5A cells in which IFN-inducible STAT activation does not
occur, STAT activation could be completely rescued by expressing
full-length IFNAR2c in the U5A cells (Fig.
2). Removal of the distal 53 residues
(R2.462) from the cytoplasmic region of IFNAR2c (R2c) had no effect on
STAT1 or STAT2 activation (Fig. 2). However, further truncation to
residue 417 (R2.417) or residue 346 (R2.346) resulted in a complete
loss of STAT1 and STAT2 activation, as measured by
IFN-dependent tyrosine phosphorylation (Fig. 2). Furthermore, substitution of all tyrosines present in the cytoplasmic domain of IFNAR2c (R2.Y-F) with phenylalanine residues, also resulted in a complete loss of STAT1 and STAT2 activation (Fig. 2). These results suggest an obligatory role for intracellular tyrosine residues
and the 417-462 region of IFNAR2c in activation of STAT1 and STAT2.
Furthermore, the distal 53 residues of IFNAR2c, which contain a
potentially phosphorylatable tyrosine residue at position 512, are
apparently not required for STAT activation.
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Upon IFN stimulation, STAT1 and STAT2 assemble to form the ISFG3
transcription complex (27). Formation of other
IFN-dependent STAT containing transcription complexes also
occurs, such as those binding to the m67 c-sis-inducible
element (SIF) present in the promoter region of the c-fos
gene (6, 28). IFN-dependent formation of both ISGF3 (Fig.
3A) and SIF (Fig.
3B) complexes were determined for all of the IFNAR2c
truncation mutants. Formation of ISGF3 and SIF complexes were observed
in response to IFN2 or IFN1b stimulation in HT1080, R2c, and
R2.462 cell lines but not in U5A, R2.Y-F, and cells expressing the
R2.417 and R2.346 IFNAR2c truncation mutants (Fig. 3, A and
B). These results are consistent with observations
demonstrating a loss of STAT1 and STAT2 phosphorylation-activation in
the R2.Y-F and R2.417 and R2.346 IFNAR2c mutants (Fig. 2).
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In a recent report, it has been suggested that IFN-inducible STAT
complex formation and DNA binding does not necessarily correlate with
IFN-inducible transcriptional activation (29). Apparently, following
STAT-DNA binding, there is an obligatory event, which is
p38-dependent, which is required for transactivation and
transcription (29). Accordingly, we undertook experiments to determine
whether any of the mutations introduced into IFNAR2c in the
transfectants affected IFN-inducible gene induction. Specifically,
IFN-inducible gene expression for known IFN-responsive genes was
examined by TaqMan® analysis (15) and RNase protection
assays (16). As shown in Table II,
IFN-inducible R1, ISG 54, and ISG 6-16 gene expression was observed
in the HT1080, R2c, and R2.462 cell lines but not in U5A cells
expressing the R2.417, R2.346, and R2.Y-F IFNAR2c mutants. A similar
pattern of gene expression was observed using RNase protection assays
(data not shown). In all cases for which gene expression could be
measured, both IFN2 and IFN1b were capable of inducing gene
expression, although some variation in gene expression levels was
observed depending on whether IFN2 or IFN1b was used. As
expected, differential expression of R1 and ISG-54 was observed in
HT1080 cells and to some extent in the R2c and R2.462 cell lines.
Consistent with the gel shift data, IFN- and
IFN-dependent gene expression was absent in cells
expressing IFNAR2c truncation mutants R2.417 or R2.346 and IFNAR2c
lacking intracellular tyrosine residues (R2.Y-F).
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IFN-dependent gene expression leads to a number of
important cellular responses such as control of cell growth. Therefore, we examined the effects of the various IFNAR2c mutants on
IFN-dependent growth inhibitory effects as measured by
short term [3H]thymidine incorporation. Consistent with
STAT activation and gene expression studies, IFN-inducible growth
inhibition was not observed in the U5A, R2.417, R2.346, and R2.Y-F
transfectant cell lines (Fig. 4).
However, IFN stimulation of U5A cells expressing IFNAR2c (R2c) or the
R2.462 mutant did result in a strong inhibition of
[3H]thymidine incorporation (Fig. 4). A similar pattern
of antiproliferative effects was observed over a 4-5-day period (data
not shown).
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DISCUSSION |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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Studies using identical mutant human IFNAR2c variants expressed in
mouse L-929 cells have been reported previously (6, 12).
Such cells simultaneously express a heterologous combination of both
mouse and human type I IFN receptor chains in which the specific
response to human IFNs is generally dependent on the absolute species
specificity of type I IFNs. Using this approach, two IFN-regulatory
regions of IFNAR2c have been reported. These include an IFN response
region (IBR) located between residues 417-462 (30) and a distal
negative regulatory domain (31). Furthermore, a STAT2 binding site was
mapped to the 404-462 region of IFNAR2c using glutathione
S-transferase fusion proteins encoding different regions of
the intracellular domain (6).
The existence of an IFN response region (IBR) or distal
negative regulatory domain was not observed in the current study in
human cells due to a complete loss of receptor function in IFNAR2c
mutants truncated at residue 417. This is in contrast to results
obtained when identical IFNAR2c truncation mutants were stably
expressed in mouse L929 cells. In this case,
IFN2-dependent antiviral effects and detectable STAT2
and STAT1 tyrosine phosphorylation were observed in mouse cells
expressing IFNAR2c truncated at residues 417 or 346. Furthermore, a
negative regulatory effect on cell growth as measured by
[3H]thymidine incorporation was not observed for any of
the IFNAR2c mutants analyzed in the present study. Only IFNAR2c and the
R2.462 truncation mutant expressed in U5A cells were capable of
producing an inhibition of [3H]thymidine incorporation
upon stimulation with type I IFN. Therefore, a complete loss of
receptor function occurs in U5A cells expressing IFNAR2c mutants
R2.417, R2.346, and R2.Y-F as measured by STAT1 and STAT2 activation,
ISGF3/SIF complex formation, gene expression (R1, ISG 54, ISG
6-16), and antiproliferative activity. A differential induction of an
antiviral state was previously reported for human IFN and IFN2 on
murine cells expressing the R2.417 or R2.346 IFNAR2c truncation mutant
and wild type IFNAR1 (30). However, this observed antiviral activity
did not correlated with impaired Janus kinase, STAT1, and STAT2
activation or ISGF3 complex formation. Therefore, the induction of an
antiviral state in these cells by human IFNs is likely to require a
functional JAK/STAT activation pathway, which is absent in U5A cells
expressing similar IFNAR2c truncation mutants.
Our data confirm previous results demonstrating the requirement of the 417-462 region of IFNAR2c for STAT activation and receptor function. However, in human cells, this region is absolutely required for receptor function and cannot be compensated for by additional STAT binding sites on either receptor chain. It is likely that, even though in U5A cells expressing IFNAR2c mutants, TYK2 and JAK1 activation occurs in response to type I IFNs, the inability of R2.417, R2.346, and R2.Y-F to induce STAT phosphorylation is due to the inability of these mutants to bind STATs or correctly present them as substrates for activated JAKs. The lack of any STAT activation in human U5A cells, which express IFNAR1, confirms that IFNAR1 on its own is unable to induce downstream signaling events such as STAT activation. In addition, it is interesting to note that, even though the 417-462 region of IFNAR2c was demonstrated to be critical for STAT1 and STAT2 phosphorylation, there are no tyrosine residues within this region. This confirms that the interaction of STATs with this site is independent of tyrosine phosphorylation. Furthermore, the distal tyrosine at residue 512 (Tyr512) is not present in the R2.462 IFNAR2c truncation mutant, demonstrating that Tyr512 appears not to be required for IFN-dependent STAT1 and STAT2 activation, transcription complex formation, gene expression, or antiproliferative effects.
Species differences in STATs and JAKs have been documented (25) and may
lead to variations in the way mouse and human cells couple
IFN-dependent receptor activation to gene expression.
Indeed, the differences in receptor function observed using IFNAR2c
mutants expressed in either mouse or human cells is unclear but may be partly due to such species differences. However, it is clear from studies using either human or mouse cells that both
phosphotyrosine-dependent and -independent sites exist
within the intracellular domain of IFNAR2c, which couple downstream
signaling to type I IFN receptor activation. Clearly, our data
demonstrate for the first time that differences exist in the manner in
which the human and murine IFNAR2c influences IFN-dependent
STAT activation. It will now be necessary to determine which
phosphotyrosine residues in IFNAR2c are critical for IFN signaling and
what role they play in regulating differential type I IFN signaling and
gene expression in human cells.
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ACKNOWLEDGEMENTS |
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We thank George Stark and Ian Kerr for making available the U5A cells and Tao Wei for helping to perform RNase protection assays.
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FOOTNOTES |
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* This work was supported in part by a Medical Research Council of Canada grant (to E. F.) and by National Institutes of Health Grants CA 55079 and GM54709 (both to O. R. C.) and 2PO1 62220, Project 3 (to R. M. R.).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. Section 1734 solely to indicate this fact.
** To whom correspondence should be addressed: Dept. of Immunology, 15049 San Pablo Ave., Berlex Biosciences, Richmond, CA 94804. Tel.: 510-669-4043; Fax: 510-669-4246; E-mail: ed_croze@berlex.com.
Published, JBC Papers in Press, May 23, 2000, DOI 10.1074/jbc.M002518200
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ABBREVIATIONS |
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The abbreviations used are:
IFN, type I
interferon;
IFNAR1, human type I interferon receptor chain 1;
IFNAR2c, human type I interferon receptor chain 2;
ISGF3, interferon-stimulated gene factor 3;
EMSA, electrophoretic mobility
shift assay;
STAT, signal transducer and activator of transcription;
SIF, c-sis-inducible factor;
JAK, Janus kinase;
PAGE, polyacrylamide gel electrophoresis.
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REFERENCES |
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TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES
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