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PHAGOCYTES
From the Laboratory of Molecular Immunoregulation,
National Cancer Institute-Frederick Cancer Research and Development
Center, Frederick, MD.
Polymorphonuclear leukocytes (PMNLs) are thought to be terminally
differentiated, short-lived, and unable to actively synthesize new
proteins or to interact with T cells. In the current study, it was
found that PMNLs incubated with supernatants of phytohemagglutinin (PHA)-stimulated peripheral blood mononuclear cells (PHA-sup) expressed
high levels of CCR6 mRNA. Neutralization with IgG against several
cytokines revealed that tumor necrosis factor (TNF)- Polymorphonuclear leukocytes (PMNLs) are the most
abundant white blood cells and comprise approximately two thirds of
circulating leukocytes in humans. In response to inflammatory stimuli,
PMNLs immediately migrate to inflamed tissues and contribute to the clearance of pathogens by phagocytosis and by releasing cytotoxic compounds. Circulating PMNLs are thought to be terminally
differentiated, short-lived, unable to actively synthesize new
proteins, and unable to interact with T cells. However, it is now known
that PMNL survival can be greatly extended in the tissues after
exposure to microenvironmental signals involved in infection and
immunity.1-3 Furthermore, PMNLs are capable of
synthesizing and releasing immunoregulatory cytokines after activation
with inflammatory cytokines.3 Low-level expression of
major histocompatibility complex class II molecules was also observed
in PMNLs after in vitro activation with granulocyte
macrophage-colony-stimulating factor (GM-CSF), interferon (IFN)- We recently reported that PMNL expressed and produced the
CC-chemokine monocyte chemoattractant protein-1 (MCP-1) after in vitro
culture with crude culture supernatants of phytohemagglutinin (PHA)-stimulated peripheral blood mononuclear cells (PBMCs) (designated as PHA-sup).8 Unlike other chemokines, such as IL-8 and
MIP-1s, whose mRNA could be induced in PMNLs within 1 hour of
stimulation, the expression of MCP-1 was always delayed, and at least 9 hours of stimulation were necessary to detect significant increases in
MCP-1 mRNA. Early protein synthesis and tyrosine phosphorylation were
involved in the expression of MCP-1. Expression of MCP-1 in PMNL
appears to be regulated by a novel mechanism that consists of 2 steps:
priming with an unidentified factor that alters the responsiveness of
PMNLs to TNF- To better understand the molecular events occurring in
cytokine-stimulated PMNLs and to identify the functions PMNLs may
acquire, we recently screened approximately 7000 human genes with a
cDNA microarray (unpublished) and found that the CC-chemokine receptor CCR6, which is exclusively expressed in immature dendritic cells (DCs),
T cells, and B cells, was one of the highly up-regulated genes in
PHA-sup-stimulated PMNLs. This finding prompted us to further
investigate whether PMNLs could undergo phenotypic and functional
changes similar to those observed during the maturation of DCs. In the
current study, we demonstrate that human PMNLs activated with PHA-sup,
or cytokines such as TNF- Reagents
Preparation of PMNLs
Activation of PMNLs and Northern blot analysis Fifteen million PMNLs were cultured in 3 mL RPMI 1640 supplemented with 10% FCS in the presence or absence of appropriate stimulants in 6-well plates (Costar, Cambridge, MA). Total RNA was extracted from each cultured PMNL using TRIZOL Reagent. Northern blot analysis was performed as previously described.10 Blots were hybridized with human CCR6 or -actin cDNA probe labeled with [ -32P]dCTP. The
intensity of mRNA expression was quantified by densitometry.
Chemotaxis assay Chemotaxis assay was performed by using a 48-well microchemotaxis chamber (Neuroprobe, Cabin John, MD). After incubation under appropriate conditions, PMNLs were rinsed 3 times and added to the upper wells of the chambers that were separated from the lower wells containing chemoattractants by a polycarbonate membrane with 5-µm diameter pores. The number of PMNLs migrating through the pores during a 60-minute incubation was counted. Results were presented as chemotactic index denoting the fold increase of cell migration in response to stimulants over control.Receptor-ligand binding assay Ten million PMNLs were incubated with 125I-labeled LARC with increasing amounts of unlabeled LARC for 1 hour at room temperature. Cells were then centrifuged through 0.8 mL of 10% sucrose cushion in microcentrifuge tubes. The tips of the tubes containing cell pellets were incised, and cell-associated radioactivities were counted by a gamma counter. Binding data were analyzed by the LIGAND program.11FACS analysis PMNLs were first washed 3 times with PBS supplemented with 1% FCS and 0.02% NaN3, and then they were incubated with each primary antibody or control IgG at room temperature for 1 hour. Cells were washed 3 times and incubated with FITC-conjugated rabbit antimouse IgG for 30 minutes and fixed with 1% paraformaldehyde in PBS, and the expression of antigen was analyzed by a FACScan flow cytometer (Becton Dickinson, San Jose, CA).In situ hybridization Cytospin preparations of PMNLs were subjected to nonradioactive in situ hybridization described previously with some modifications.12 Briefly, digoxigenin-labeled antisense and sense cRNA probes for human CCR6 were synthesized using the DIG RNA labeling kit (Boehringer Mannheim). Cells fixed in 4% paraformaldehyde were treated with proteinase K, denatured with 0.2 N HCl, acetylated with 0.1 mol/L triethanolamine and 0.25% acetic anhydride, and hybridized for 16 hours at 50°C with In Situ Hyb Buffer containing cRNA probes (20 ng/30 µL). After hybridization, the cells were washed with 2 × SSC and 50% formamide and treated with RNase A for digestion of unhybridized probes. Hybridized probe was detected immunologically using anti-digoxigenin-fluorescein Fab fragments under a fluorescein microscope.Reverse transcription-polymerase chain reaction Reverse transcription-polymerase chain reaction (RT-PCR) was performed using Superscript II 1 Step RT-PCR System (Life Technologies) with total RNA extracted from fresh or stimulated PMNLs. Primers used were 5'-CTGTGGACAAAGCCAACTTG-3' and 5'-ACGTTCTCTGTAGTCTCTGG-3' for HLA-DR-chain; 5'-CTCCGAAGATGTGGACTTGC-3' and
5'-ATGCCAGCTTTAGAAAAATC-3' for CD83; and 5'-GCAGGACCAGGAAAACTTGG-3' and
5'-AGAAAGGTGAAGATAAAAGC -3' for CD86.
TNF- (lane 5), but not IFN- (lane
6) or GM-CSF (lane 7). The addition of all 3 IgGs did not further
increase the inhibitory effect obtained by anti-TNF- IgG (lane 8).
The addition of each IgG did not induce CCR6 mRNA expression (lanes
9-11). These results indicated that TNF- contained in the PHA-sup
played a major role in the induction of CCR6 mRNA expression.
The effect of several recombinant cytokines on the CCR6 mRNA expression
was next investigated. As shown in Figure 1, panel B, a high level of
CCR6 mRNA was detected in PMNLs stimulated with TNF- The effects of TNF-
A study of the kinetics of the response showed that the peak CCR6 mRNA
expression was detected at 3 hours and was sustained up to 16 hours
after activation with TNF-
125I-labeled LARC specifically binds to PMNLs
activated with TNF- and IFN-, there
was a significant binding of 125I-LARC that was
competitively inhibited by the addition of increasing amounts of
unlabeled LARC, but not by IL-8 or MCP-1 (Figure
4A). The estimated equilibrium
dissociation constant (Kd) of LARC-PMNL binding
and the number of binding sites were 1.6 nmol/L and 160 sites per cell,
respectively (Figure 4B). There was no specific binding of
125I-LARC after overnight incubation, suggesting that the
cell-surface expression of CCR6 was transient (data not
shown).
Cytokine-activated PMNLs dose-dependently migrate to LARC To examine whether CCR6 on cytokine-activated PMNLs was functional, migration of PMNLs to LARC was evaluated by an in vitro chemotaxis assay. Freshly isolated PMNLs responded to IL-8 or fMLP but did not respond to any concentrations of LARC (data not shown). However, PMNLs activated with the PHA-sup (Figure 5A), TNF- and GM-CSF (Figure 5B), or
TNF- and IFN- (Figure 5C) for 6 hours exhibited a potent
migration toward LARC in a dose-dependent manner. There was no
significant decrease in the number of migrating cells at 10 µg/mL
LARC (data not shown). In contrast, PMNLs cultured overnight in the
presence of either PHA-sup or a combination of TNF- and GM-CSF did
not migrate toward LARC, suggesting that the expression of CCR6 was
transient (Figure 5A,B). LARC did not induce calcium flux in PMNLs at a
concentration range up to 10 µg/mL after 6 hours of incubation with
the PHA-sup (data not shown).
TNF- , and IFN-
induced higher levels of CD40 and CD83 and a high level of HLA-DR, but no significant CD86 expression (data not shown).
Expression of CCR7 mRNA is not induced in PMNLs We additionally examined whether cytokine-activated PMNLs express the CC-chemokine receptor CCR7 that has been reported to be expressed on mature DCs. There was no detectable CCR7 mRNA expression in activated PMNLs by RT-PCR up to 4 days (data not shown), supporting that the differentiated PMNL are distinct from "mature" DCs.
The current study has, for the first time, clearly shown that
PMNLs could be induced to express functional CCR6 after activation with
selected cytokines. TNF- There is considerable evidence that the expression of CCR6 on DCs
occurs during an earlier stage of maturation and accounts for the
trafficking of immature DCs to inflammatory sites where LARC is
produced.15 CD34+ progenitor cell-derived DCs
expressed CCR6 during in vitro culture by day 6, but the expression of
CCR6 was undetectable at day 14.16 Immature DCs generated
from monocytes in the presence of GM-CSF, IL-4, and TGF- It was previously reported that IFN- The capacity of certain chemokines to recruit and activate certain
leukocyte populations can be altered by up- or down-regulating the
expression of chemokine receptors due to proinflammatory cytokines produced during inflammation. For example, PMNLs from rats with chronic
inflammatory vasculitis expressing CCR1 and CCR2 migrated toward
MCP-1.18 CCR1 and CCR3 expressed on IFN- Oehler et al22 previously reported that
lactoferrin-positive immediate precursors of end-stage PMNLs could be
driven to acquire characteristics of DCs, including HLA-DR, CD40, CD80, and CD86, after activation with GM-CSF, TNF- Another important feature of mature DCs is to present antigens to T
cells. PMNLs activated with either PHA-sup or a combination of TNF- The importance of PMNLs in the development of delayed-type
hypersensitivity (DTH) was previously demonstrated in vivo. Depletion of PMNLs inhibited the infiltration of monocytes and lymphocytes in a
murine model of DTH.23,24 Injection of anti-IL-8 antibody inhibited the development of DTH in a rabbit DTH model.25
In a rat DTH model, MCP-1, an important chemokine regulating the infiltration of monocytes in DTH, was detected by immunohistochemistry in early infiltrating PMNLs, and neutralization of MCP-1 activity with
anti-MCP-1 antibody inhibited the development of DTH.26 In support of these observations, we previously reported that human
PMNLs could be induced to express and produce MCP-1 in
vitro.8 We recently suggested that the priming of PMNLs
with a product(s) of PHA-stimulated PBMCs could functionally change the
ability of PMNLs to express MCP-1.9 In the current study,
we have shown further evidence indicating the capacity of PMNLs to
acquire phenotypic and functional changes after activation with
selected cytokines, including TNF-
We thank Dr Joost J. Oppenheim for his encouragement and invaluable comments throughout this study. We also thank Ms Nancy Dunlop for her technical assistance.
Submitted April 26, 2000; accepted August 3, 2000.
Supported by the Intramural Research Support Program, SAIC (Frederick, MD) (W.-H.G.).
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: Teizo Yoshimura, Laboratory of Molecular Immunoregulation, National Cancer Institute-Frederick Cancer Research and Development Center, Bldg 559, Rm 1, Frederick, MD 21702; e-mail: yoshimur{at}mail.ncifcrf.gov.
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© 2000 by The American Society of Hematology.
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Abstract
Introduction
8
mol/L) and IL-8 (100 ng/mL) were used as positive controls.
