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Blood, Vol. 95 No. 5 (March 1), 2000:
pp. 1810-1818
PHAGOCYTES
From the The Phagocyte Research Laboratory, Department of Medical
Microbiology and Immunology, and Department of Oral Microbiology,
University of Göteborg, Göteborg, Sweden, and DBMS/BBSI
(UMR 314, CEA/CNRS) CEA-Grenoble, France.
A D-methionine-containing peptide,
Trp-Lys-Tyr-Met-Val-D-Met-NH2 (WKYMVm), featuring a unique
receptor specificity was investigated with respect to its ability to
activate neutrophil effector functions. The peptide was found to be
more potent than the N-formylated peptide N-formyl-Met-Leu-Phe (fMLF)
at inducing neutrophil chemotaxis, mobilization of neutrophil
complement receptor 3 (CR3), and activation of the neutrophil
NADPH-oxidase. The fact that binding of fML[3H]F was
inhibited by both fMLF and WKYMVm suggests that N-formyl peptide
receptor (FPR) is shared by these peptides. However, the neutrophil
response induced by the WKYMVm peptide was insensitive to the fMLF
antagonists, cyclosporin H, and Boc-FLFLF that specifically block the
function of the FPR. These results suggest that even though WKYMVm may
bind FPR the cells are activated preferentially through a receptor
distinct from the FPR. Using transfected HL-60 cells expressing either
the FPR or its neutrophil homologue FPRL1, also referred to as
LXA4R because it has been shown to bind lipoxin A4, we show that WKYMVm is about 300-fold more active at
mobilizing intracellular calcium through FPRL1 than through FPR. The
WKYMVm activates FPRL1-expressing cells in a cyclosporin H-independent manner with an EC50 of around 75 pmol/L, whereas it
activates FPR-expressing cells with an EC50 of around 25 nmol/L. The observation that exudated cells are primed in their
response to WKYMVm suggests that FPRL1/LXA4R like FPR is
stored in mobilizable organelles.
(Blood. 2000;95:1810-1818)
The human neutrophils play a key role in the innate
immune response to infection. They act at inflammatory sites, which
they reach after targeting and extravasation from the peripheral blood stream. The extravasation process is induced by different
chemoattractants.1-3 These chemoattractants are recognized
by G-protein-coupled cell surface receptors, and the second messengers
generated by the dissociated G By screening a number of random oligopeptide sequences, Seo and
coworkers16,17 recently identified a new group of peptides with a unique receptor specificity. These are hexapeptides with the
consensus sequence XKYX(P/V)M that bind to a G-protein-coupled receptor in several leukocyte cell lines, resulting in activation of
phospholipase C.16,17 Substitution of the L-methionine at the carboxy-terminus with a D-methionine markedly increased the potency
of the peptides17 and the D-methionyl-containing peptide was shown to activate the NADPH-oxidase in peripheral blood
neutrophils, provided that the cell cytoskeleton was first disrupted by
cytochalasin B.
The aim of this study was to further investigate the biologic
activities of the hexapeptide Trp-Lys-Tyr-Met-Val-D-Met-NH2 (WKYMVm) in relation to the function of human neutrophils. We found
that the peptide is chemotactic for neutrophils, that it induces
secretion of granule constituents and subsequently mobilization of
adhesion molecules to the cell surface, and that it is a potent activator of the NADPH-oxidase. The receptor activated by WKYMVm was
found to be identical to the formyl peptide-like receptor, FPRL1,
earlier shown to recognize lipoxin A4 and being referred to
as the lipoxin A4 receptor.3,18
Isolation of human neutrophils
Peptides and peptide receptor antagonists
Receptor binding Receptor binding of fML[3H]F was determined by centrifugation of cells through an oil layer as described earlier.23 In short, cells were allowed to bind fML [3H]F (final concentration, 2 × 10 8 mol/L) in the presence or absence of
nonradioactive peptides (fMLF or WKYMVm) for 15 minutes at 4°C.
These cell suspensions were then placed on a mixture of dibutylphtalate
and dinanylphtalate (10:3 v/v) in 250 µL Eppendorf tubes. The cells
were separated from nonbound peptide by centrifugation
(9000 × g for 30 seconds), and the tips of the tubes containing
the cells were cut off and put into scintillation vials.
Neutrophil chemotaxis A modified version of the technique described by Agace and coworkers24 was used to determine neutrophil chemotaxis.25 In short, epithelial cells (KB cells) were cultured in Dulbecco's modified Eagle's medium (GIBCO, UK) supplemented with 200 mmol/L L-glutamine, fetal calf serum, and 100 mg/mL penicillin/streptomycin. Subcultivation was performed twice a week and cells used in the experiments were never older than 25 passages. The KB cells were suspended in culture medium (0.7 × 105 cells/200 µL) and seeded on inverted Transwell inserts (Costar, Cambridge, MA; 12 mm membranes with a pore diameter of 3 µm). The cells were allowed to attach onto the membrane and after 2 days of incubation the cell layers were confluent.Neutrophil NADPH-oxidase activity The NADPH-oxidase activity was determined using a luminol/isoluminol-enhanced chemiluminescence (CL) system.27 The CL activity was measured in a 6-channel Biolumat LB 9505 (Berthold Co. Wildbad, Germany), using disposable 4-mL polypropylene tubes with a 0.90-mL reaction mixture containing 1 to 2 × 105 neutrophils. The tubes were equilibrated in the Biolumat for 5 minutes at 37°C, after which the stimulus (0.1 mL) was added. The light emission was recorded continuously. To quantify intracellularly and extracellularly generated reactive oxygen species, respectively, 2 different reaction mixtures were used. Tubes used for measurement of extracellular release of superoxide anion contained neutrophils, horseradish peroxidase (HRP; a cell impermeable peroxidase; 4U), and isoluminol (a cell impermeable CL substrate; 2 × 105 mol/L).27 By a direct
comparison of the superoxide dismutase (SOD) inhibitable reduction of
cytochrome C and SOD inhibitable CL, 7.2 × 107 cpm
were found to correspond to a production of 1 nmol of superoxide (a
millimolar extinction coefficient for cytochrome C of 21.1 was used;
details about the CL technique are given by Lundqvist and
Dahlgren27). Tubes used for measurement of intracellular generation of reactive oxygen species contained neutrophils, SOD (a
cell impermeable scavenger for O2; 50 U), catalase (a cell impermeable scavenger for
H2O2; 2000 U), and luminol (a cell permeable CL
substrate; 2 × 105 mol/L).
Mobilization of complement receptor 3 Mobilization of subcellular organelles was followed by measuring the exposure of complement receptor 3 (CR3) on the neutrophil surface. Cells were labeled with phycoerythrin-conjugated monoclonal antibodies specific for CD11b (Becton Dickinson Clone 12 cat.no 347550; 10 µL to a cell pellet of 106 cell), and examined by FACScan (Becton Dickinson, Mountain View, CA).28Subcellular fractionation Subcellular fractionation was performed by the method described by Borregaard et al.29 In short, neutrophils were resuspended in relaxation buffer and disintegrated by nitrogen cavitation (Parr Instrument Company, Moline, IL). The postnuclear supernatant was centrifuged on a Percoll gradient of 14 mL solution with a density of 1.05 g/mL, overlaying 14 mL of a solution with a density of 1.12 g/mL. The gradients were collected in 1.5 mL fractions by aspiration from the bottom of the centrifuge tube and the localization of subcellular organelles in the gradients was determined by marker analysis of the fractions. Alkaline phosphatase (ALP) activity was measured by hydrolysis of p-nitrophenyl phosphate (PNPP; 3.5 mmol/L) at pH 10.5 in a sodium-barbital buffer. Subcellular fractions were added to a buffer solution with or without Triton X-100 (0.2% final concentration) and containing the substrate; the samples were then incubated at 37°C for 45 minutes, hydrolysis of the substrate was determined as an increase in absorbance at 410 nm, and the mobilization of the secretory vesicles was determined as a loss in ALP latency (difference in ALP activity in the presence and absence of detergent30). Vitamin B12-binding protein was determined with the cyanocobalamin technique.31 Gelatinase was measured using an enzyme-linked immunosorbent assay (ELISA) method (the antibodies used were a kind gift from Drs Lars Kjeldsen and Niels Borregaard, Copenhagen) and myeloperoxidase (MPO) was determined either by an ELISA assay or from the 472-nm peak of reduced-minus-oxidized difference spectra.29,32Neutrophil priming Two different protocols were used for mobilization of neutrophil subcellular organelles to the cell surface. The first cell population was merely incubated at 22°C for 60 minutes without additive.21,32 The second cell population was subjected to stimulation by the calcium ionophore ionomycin. After preincubation of the neutrophils at 37°C for 5 minutes, ionomycin (5 × 107 mol/L final concentration) was
added and the incubation was continued for 5 minutes. The cell
populations were then sedimented by centrifugation and the supernatants
were collected for marker analysis (described above). The pellet was
suspended in KRG, washed once to remove any prestimulating agent,
resuspended to 1 × 107 cells/mL in KRG or
relaxation buffer, and put on ice until use.
Stable expression of formyl peptide receptor and formyl peptide-like receptor in HL-60 cells The pEF-FPR and pEF-FPRL1 expression plasmids were constructed in the following way: The cDNA sequence encoding a FLAG-tagged version of formyl peptide receptor (FPR) was excised from pcDNA3.1 by Nhe I and Xba I, and that encoding FPRL1 was excised by Xba I from CDM8. Inserts were ligated into the pEF-neo plasmid cleaved by Xba I.33 Transfection of HL-60 cells was performed by electroporation with a Bio-Rad Gene Pulser apparatus, according to a slightly modified version of the technique described by Tonetti et al.34 In brief, 20 µg of supercoiled plasmid DNA in TE 10 mmol/L Tris-HCl,1 mmol/L EDTA, pH 8.0 were mixed with 107 cells in 0.5 mL of phosphate-buffered sucrose (272 mmol/L sucrose, 7 mmol/L Na2HPO4, pH 7.4). Cells were electroporated with a pulse of 250 V for 18 to 20 ms. Control cells were transfected in the same conditions with the pEF-neo plasmid encoding CXCR2 (the IL-8 receptor). After electroporation, cells were allowed to recover in 20 mL of culture medium for 48 hours before selection in a medium containing G418 (1 mg/mL). The G418 resistant transfected clones were obtained by limited dilution into 24-well microtiter plates and positive clones were identified by their ability to mobilize intracellular calcium on addition of N-formyl-Met-Leu-Phe-Lys (1µmol final concentration) and IL-8 (20 nmol), respectively.Determination of changes in cytosolic calcium HL-60 cells at the density of 1 to 3 × 106 cells/mL were washed with phosphate-buffered saline (PBS). The cell pellets were resuspended at a density of 2 × 107 cells/mL in RPMI medium without phenol red containing 0.1% bovine serum albumin (BSA) and loaded with 2 µmol Fura 2-AM for 30 minutes at 37°C. Cells were then diluted with 2 volumes of the same medium without BSA, washed once in KRG, and resuspended in RPMI medium without phenol red at a density of 2 × 107 cells/mL. Calcium measurements were carried out with a SPEX FluoroMAX fluorescence spectrophotometer (SPEX Industries, Stanmore, UK) with an excitation wavelength of 340 nm, an emission wavelength of 505 nm, and slit widths of 5 and 10 nm, respectively. Maximal and minimal fluorescence were determined in the presence of Triton X-100 and EGTA/Tris-HCl, respectively. Intracellular calcium concentrations were calculated using the following formula: [Ca++] = Kd(F Fmin)/(FmaxF)
where the Kd for Fura-2 equals 224 nmol/L.
Hexapeptide Trp-Lys-Tyr-Met-Val-D-Met-NH2 induces neutrophil chemotactic activity The ability of WKYMVm to induce chemotaxis in human neutrophils was investigated using epithelial cells grown on polycarbonate filters as a matrix over which transepithelial gradients of potential chemoattractants were formed. We found that neutrophils migrated through the filter and epithelial cell layer when WKYMVm was present in the lower compartment (Figure 1). The peptide was, thus, found to be chemotactic with a potency exceeding that of fMLF.
Hexapeptide Trp-Lys-Tyr-Met-Val-D-Met-NH2 induces NADPH-oxidase activity in neutrophils Both WKYMVm and fMLF were able to induce superoxide anion production in human neutrophils (Figure 2). The time courses of the 2 responses were very similar, but the EC50 values differed, WKYMVm being the more potent activator having an EC50 of 2 × 109 mol/L compared with
5 × 108 mol/L for fMLF.
Hexapeptide Trp-Lys-Tyr-Met-Val-D-Met-NH2-induced mobilization of neutrophil complement receptor 3 We examined to what extent WKYMVm could induce neutrophil granule mobilization by measuring the exposure of CR3 on the cell surface. Treatment with the hexapeptide at concentrations from 1 × 1012 to 1 × 107
mol/L increased the amount of CR3 on the cell surface (shown for 107 mol/L in Figure 3).
The EC50 value for WKYMVm was
5 × 1011 mol/L, whereas the corresponding
value for fMLF was 2 × 109 mol/L.
Characteristics of the receptor activated by hexapeptide Trp-Lys-Tyr-Met-Val-D-Met-NH2 The cellular responses induced by WKYMVm are in many ways similar to those induced by fMLF. To determine whether WKYMVm acts through a novel receptor or whether it interacts with a unique binding site on the fMLF receptor, we performed receptor-binding analyses and desensitization experiments.
Peptide-induced mobilization of intracellular
Ca++ in transfected HL-60 cells expressing the
formylpeptide receptor or its homolog (LXA4R/FPRL1).
In addition to the high-affinity N-formyl peptide receptor (FPR),
human neutrophils express a structurally related receptor originally
known as FPRL1. Despite its high degree of sequence similarity with the
FPR (69%), FPRL1 binds fML[3H]F with low affinity (Kd > 400 nmol/L) (reviewed in Ye and Boulay3). More recently
FPRL1 has been shown to bind lipoxin A4 with high affinity
and it is consequently referred to as LXA4R.18
To test whether FPRL1/LXA4R was able to interact with
WKYMVm, either FPR, FPRL1/LXA4R, or CXCR2 (control cells)
was stably expressed in HL-60 cells, a cell line of myeloid origin that
does not express these receptors when undifferentiated. As illustrated
in Figure 7A (inset), the formylpeptide
induced a rise in intracellular calcium in FPR expressing cells with an
EC50 of around 5 nmol/L, whereas WKYMVm had an
EC50 of around 25 nmol/L. This indicates that FPR is a
shared receptor for the 2 peptides. Interestingly, when WKYMVm was
assayed with FPRL1/LXA4R-expressing cells, it induced a
rise of intracellular calcium with an EC50 around 75 pmol/L, whereas concentrations of the formyl peptide higher than 500 nmol/L were necessary to mobilize the same level of intracellular calcium (Figure 7B, inset). The CsH was found to be inactive on FPRL1/LXA4R-expressing cells (not shown). The fMLFK was
found to be a better agonist for FPRL1 than the prototypical peptide fMLF, which was unable to trigger calcium mobilization with
concentrations lower than 1 µmol/L (data not shown). Thus, WKYMVm is
at least 6 000-fold more potent than the formyl peptide at stimulating the FPRL1/LXA4R. Neither of the 2 peptides induced a
calcium increase in transfected HL-60 cells expressing CXCR2.
Neutrophil priming
We found the D-methionine-containing hexapeptide WKYMVm to be a
potent agonist in terms of chemotactic activity, capability to mobilize
neutrophil granules/vesicles, and ability to induce a neutrophil
respiratory burst response. This peptide was first identified by Seo
and coworkers17 as a molecule that activates PLC in several
leukocyte cell lines. The details of the structure-activity relationship of the peptide was determined, and it was found that Met6 was critical for activity. This was illustrated by the fact that when Met6 was either eliminated or replaced by
glycin, the resulting peptides were inactive.17 The peptide
also depends highly on the presence of a D-methionine at its C-terminus
(introduction of an L-type amino acid, replacing the D-Met, increases
the EC50 value 100-fold17; our own unpublished
observation). Seo and coworkers17 suggested that WKYMVm is
recognized by a unique receptor. Here we bring this issue further and
determine the identity of this receptor. Cyclosporin H abrogated the
fMLF induced cellular response, whereas the WKYMVm-induced response was
unaffected. Although CsH is completely unrelated to the N-formyl
peptide, it is a potent antagonist of N-formyl peptide binding to the
FPR and of functional responses triggered by fMLF,35 and
our results, thus, support the suggestion that the WKYMVm peptide
activates neutrophils through a receptor different from the FPR.
Nevertheless, the mechanisms of activation downstream of the receptors
are very similar for these 2 peptides.
The skillful technical assistance of Lisbeth Björck is gratefully acknowledged.
Submitted March 15, 1999; accepted October 29, 1999.
The work of the Swedish group was supported by the Swedish Medical
Research Council, the King Gustaf V 80-Year Foundation, the Fredrik and
Ingrid Thuring Foundation, the Lars Hierta Foundation, the Anna-Greta
Crafoord Foundation for Rheumatological Research, the Vårdal
Foundation, and The Swedish Society of Medicine. The work of the French
group was supported by grants from the Commissariat à l'Energie
Atomique, the Centre National de la Recherche Scientifique (CNRS), and
the University Joseph Fourier.
Reprints: Claes Dahlgren, The Phagocyte Research Laboratory,
Department of Medical Microbiology and Immunology, Guldhedsgatan 10, S-413 46 Göteborg, Sweden; e-mail:
claes.dahlgren{at}microbio.gu.se.
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.
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Abstract
Introduction
and G
subunit complex activate downstream effector molecules.
