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IMMUNOBIOLOGY
From the Department of Pathology and Laboratory
Medicine, University of Wisconsin Medical School, Madison.
Granulocyte-macrophage colony-stimulating factor (GM-CSF) is
critical for promoting the long-term survival of lung- or airway-based eosinophils. Previously, we have shown that fibronectin and tumor necrosis factor Eosinophils are a major source of proinflammmatory
mediators in the airway and lung parenchyma of atopic and asthmatic
patients.1 In the asthmatic lung, normally short-lived
eosinophils become resistant to apoptosis through the autocrine
production and release of granulocyte-macrophage colony-stimulating
factor (GM-CSF).2 This process can be initiated by
engagement of many cell-surface receptors (CD9, CD32, Specifically, TNF- To better understand the signaling cascades leading to mRNA
stabilization, several studies have focused on the role of
mitogen-activated protein kinases (MAPKs). Indeed,
c-jun-NH2-terminal kinase (JNK) activation was required for
interleukin 2 (IL-2) and IL-3 mRNA stabilization in T-cell or mast cell
lines.10,11 Here, we investigated if MAPKs (ERK, p38, or
JNK) were responsible for GM-CSF mRNA stabilization in TNF- Subjects and eosinophil preparation
Eosinophils (typically > 98% pure) were purified by using a negative
immunomagnetic procedure as previously described.12 After
isolation, eosinophils were maintained in RPMI 1640 medium, 10% fetal
calf serum, and 50 µg/mL gentamicin (all from Gibco Life
Technologies, Grand Island, NY), at 37°C in a 5% CO2 environment.
Reagents and eosinophil activation
Recombinant human TNF- Cell lysates and Western blotting Following incubation, the cells were pelleted and resuspended in the lysis buffer (20 mM Tris, 137 mM NaCl, 1 mM EDTA, 0.1 mM sodium orthovanate, 10 mM sodium fluoride, 10 mM -glycerol phosphate and
protease inhibitors, pH 7.4, 1% Triton X-100, 0.25% deoxycholate, and
0.1% sodium dodecyl sulfate [SDS]), as previously described.13 The cells were passed 10 times through a
29-gauge needle and incubated on ice for 10 minutes. The eosinophil
lysates were centrifuged at 12 000g for 2 minutes to remove
the insoluble material, and the supernatants were stored at  80°C
before immunoblotting. The primary antibodies were detected with an
antirabbit horseradish peroxidase-conjugated secondary antibody and
developed by using the enhanced chemiluminescence system (Amersham,
Piscataway, NJ). The signals obtained by autoradiography were
quantified on an AlphaImager 2200 analysis system (Innotech, San
Leandro, CA).
Plasmid constructions, mRNA transfection, and Northern blotting Complementary DNA (cDNA) coding for human GM-CSF was obtained from the American Type Culture Collection (Rockville, MD). The plasmid for in vitro, wild-type GM-CSF mRNA synthesis has been described previously.14Particle-mediated gene transfer of in vitro-transcribed mRNAs into cultured cells was performed by using the Accell Gene-Gun (Powerject, Madison, WI), as previously described.12 At indicated times, cells were pelleted and lysed in TRIreagent (Molecular Research Center, Cincinnati, OH), and total RNA was quantitatively isolated and analyzed by Northern blotting with a radioactively labeled GM-CSF or actin cDNA probes as described previously.12 GM-CSF mRNA signals were normalized to those for actin mRNA to accommodate any differences in the extraction, gel loading, and transfer of total RNA. After stringent washing at 50°C for 5 minutes with 0.1 × sodium chloride/sodium citrate and 0.1% SDS, the blots were quantitated by phosphorimaging (Model 445SI; Molecular Dynamics, Sunnyvale, CA). MEK1(E) or MKK3b(E) transduction The coding region of constitutively active human MAPKK (MEK1(E) or MKK3b(E))15,16 were generously provided by Jiahui Han, La Jolla, CA. The full-length coding region was cloned into pTatHA9,17,18 coding for a fusion protein containing from N to C terminus: 6-histidine, Tat translocation sequence, hemagglutinin epitope, and MEK1(E) or MKK3b(E) that was expressed in BL21 cells. As previously described,9 expressing bacterial cultures were dissolved in 8 M urea, 50 mM Tris pH 8.0, 150 mM NaCl, sonicated, and centrifuged at 15 000g. Cleared lysate was mixed with NiNTA resin (Qiagen, Valencia, CA) in the presence of 10 mM imidazole, and His-tagged protein was allowed to bind. The resin was washed 3 times with 8 M urea, 50 mM Tris pH 8.0, 150 mM NaCl, 10 mM imidazole. Protein was eluted with 1 M imidazole, 50 mM Tris pH 8.0, 150 mM NaCl and dialyzed against phosphate-buffered saline. Protein was more than 90% pure by Coomassie-stained SDS-polyacrylamide gel electrophoresis analysis. Tat fusion protein (10 nM; TatMEK1(E) or TatMKK3b(E)) was added to 8 × 106 cells for 2 hours at 37°C that were then transfected with the Gene-Gun as described above. After washing, GM-CSF mRNA stability (half-life time) was determined by Northern blot as described above, and for survival experiments the cells were cultured for 1 hour after transduction at 1 × 107 cells/mL, diluted 1:10, and cultured for 4 days. Viability was determined as previously described.19Statistical analysis Results were expressed as mean ± SD or SEM. Statistical analysis was performed by using paired and unpaired Student t tests. Correlation data were analyzed for statistical significance by using the Pearson test. P values < .05 were considered as statistically significant.
Eosinophils treated with TNF-  plus Fn showed increased GM-CSF mRNA accumulation, stability, and GM-CSF protein production.2 In an effort to understand the signaling cascades underlying these effects, we evaluated MAPK
activation. These kinases were essential for IL-2 and IL-3 mRNA
stabilization in T and mast cells.10,11 As shown in Figure 1A,B, the treatment of pbeos with TNF-
plus Fn activated ERK and p38 but not JNK, which was slightly
phosphorylated in resting eosinophils. Of note, kinetic experiments
showed that ERK and p38 reached their activation maxima between 5 and
60 minutes after stimulation, whereas JNK phosphorylation was unchanged
(data not shown), consistent with another report.20
PD98059 completely abrogated ERK phosphorylation but had no significant
effect on the quantity of phosphorylated p38 (Figure 1A,B, lane 5). In
contrast, U0126, another specific ERK inhibitor, prevented ERK and p38
phosphorylation equally well (not shown). Treatment of pbeos with
TNF- alone predominantly activated p38, although some phosphorylated
ERK was detected, whereas Fn alone had the reverse effect, mostly activating ERK and only slightly p38 (Figure 1A-B). These data are
consistent with prior studies in eosinophils.21,22 Thus, it is likely that Fn or TNF- activated the appropriate pbeos pathways in our hands and suggested that selective MAPK activation might control GM-CSF mRNA stability.
ERK activation was correlated with GM-CSF mRNA stabilization To connect MAPK with mRNA decay, we correlated GM-CSF mRNA stability in pbeos after exposure to TNF-, Fn, or both agents with
the level of MAPK activation (Figure 2).
Clearly, GM-CSF mRNA stability was highly correlated with ERK
activation (r = 0.961; P < .04), whereas p38
phosphorylation was not (Figure 2; r = 0.649;
P > .35). Consistent with these data, GM-CSF mRNA never accumulated nor was stabilized in eosinophils treated with
TNF-2 that activates p38 (Figure 1).
ERK inhibitors block GM-CSF mRNA stabilization To confirm the respective roles of ERK and p38, we transfected GM-CSF mRNA into pbeos following treatments with MAPK inhibitors and TNF- plus Fn. The decay rate of exogenous GM-CSF mRNA was measured
by Northern blotting. As previously reported by our
laboratory,2 TNF- plus Fn stabilized GM-CSF mRNA in
pbeos (GM-CSF mRNA half-life = 24 minutes) (Figure
3A-B), which was completely prevented by the ERK inhibitor (PD98059) (GM-CSF mRNA half-life = 12 minutes) (Figure 3A-B), suggesting that ERK activation was necessary for GM-CSF
mRNA stabilization. The p38 inhibitor (SB203580) had an intermediate
effect, attenuating GM-CSF mRNA stabilization by approximately 50%,
suggesting that p38 contributed to GM-CSF turnover in cooperation with
ERK in the context of TNF- plus Fn-activated pbeos. However, it
remained possible that SB203580 nonspecifically affected the Erk
pathway.
ERK activation was sufficient for GM-CSF mRNA stabilization and increased eosinophil survival To demonstrate whether ERK or p38 activation was sufficient for GM-CSF mRNA stabilization, we transduced pbeos with either the constitutively active TatMEK1(E) or TatMKK3b(E) that respectively and selectively activate ERK or p38.15,16 As previously described with TatYB-1 protein,9 pbeos were incubated for 2 hours with TatMEK1(E) or TatMKK3b(E) prior to analysis of their effects on GM-CSF mRNA stability. Table 1 shows that MEK1(E) stabilized GM-CSF mRNA by more than 2-fold (t1/2 from 12 to 27 minutes; P < .048, n = 5), whereas MKK3b(E) had no effect (t1/2 from 13 to 12 minutes).
As a consequence of increased GM-CSF mRNA stability, we
anticipated eosinophil survival would be prolonged compared with
untreated controls. Therefore, viability was determined 4 days after
TatMEK1(E) or TatMKK3B(E) transduction and GM-CSF mRNA transfection. As
previously described12 GM-CSF mRNA transfection increased
eosinophil in vitro survival at 4 days from about 10% for control
eosinophils to approximately 30%. The survival of
TatMEK1(E)-transduced cells was increased by an additional 35% over
cells solely transfected with GM-CSF mRNA that was statistically
significant as calculated by the paired Student t test
(P < .014). Consistent with its failure to alter GM-CSF
mRNA stability, TatMKK3b(E) had no significant effect on eosinophil
survival (Figure 4;
P = .184) compared with GM-CSF mRNA-transfected controls.
Finally, cells transfected but then transduced with Tat
In this present study, we have investigated signaling
pathways that mediate GM-CSF posttranscriptional regulation in
eosinophils after TNF- Most of the studies analyzing the role of MAPK on mRNA stability
have used transformed cell lines (Jurkat, Hela, THP-1, fibroblastlike, or mast cell-like) as models. These studies have generally implicated p38 or JNK as critical kinases.10,11,28-32 ERK has,
however, been linked to macrophage inflammatory protein-2 or nucleolin mRNA stability in fresh rat peritoneal neutrophils or human peripheral blood mononuclear cells, respectively.33-35 Whether mRNA
regulation in primary cells, including eosinophils specifically,
depends on ERK phosphorylation remains unclear. Many previous studies have shown ERK activation as a consistent event after in vitro activation of eosinophils. For example, eotaxin induced both ERK and
p38 activation in eosinophils, whereas JNK was constitutively phosphorylated.20 Similarly, IL-5 activated both MAPK (ERK
and p38),36,37 whereas guinea pig eosinophil activation
with leukotriene B4 or human eosinophil adhesion to Fn was rapidly
followed by only ERK phosphorylation.22,38 Macrophage
inflammatory protein-3 The additive effects of TNF- Previously, we demonstrated that TNF- Our data also represent an important link in understanding how GM-CSF mRNA and other cytokine mRNAs are stabilized on cell activation. This process likely involves several ARE-specific binding proteins, including HuR, hnRNP A/C, nucleolin, and YB-1.9,35,44,45 These activities likely target the ARE and modify the recognition of labile cytokine mRNAs by the decay machinery. However, despite a common 3' untranslated ARE, GM-CSF and IL-2 mRNA stability are dependent on ERK/p38 or JNK, respectively. This dependency suggests that novel effectors must also be involved that are differentially regulated by these distinct MAPKs.
We thank the other members of the SCOR-asthma group, particularly Julie Sedgwick for providing pbeos and Mary Ellen Bates for her assistance with the MAPK analyses. We also thank Beth Capowski and Syrus Soltaninassab for their assistance for Tat protein production.
Submitted October 26, 2001; accepted January 24, 2002.
Supported by Project 5 of SCOR-asthma-P50HL56396 from the National Institutes of Health (J.S.M.).
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: James S. Malter, Department of Pathology and Laboratory Medicine K4/812-CSC, University of Wisconsin Hospital and Clinic, 600 Highland Ave, Madison, WI 53792; e-mail: jsmalter{at}facstaff.wisc.edu.
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© 2002 by The American Society of Hematology.
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  J. A. Corcoran, W.-L. Hsu, and J. R. Smiley Herpes Simplex Virus ICP27 Is Required for Virus-Induced Stabilization of the ARE-Containing IEX-1 mRNA Encoded by the Human IER3 Gene J. Virol., October 1, 2006; 80(19): 9720 - 9729. [Abstract] [Full Text] [PDF]
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fibronectin-activated peripheral blood eosinophils
Top
Abstract
Introduction
RII (CD32) pivotally regulates survival of human eosinophils.
J Immunol.
1999;162:4253-4259