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Blood, Vol. 96 No. 3 (August 1), 2000:
pp. 840-845
CHEMOKINES
From the Intramural Research Support Program, Laboratory of
Molecular Immunoregulation, Division of Basic Science, National Cancer
Institute-Frederick Cancer Research and Development Center, Frederick,
MD.
Liver-expressed chemokine (LEC) is an unusually large CC chemokine,
which is also known as LMC, HCC-4, NCC-4, and CCL16. Previously, LEC
was shown to induce leukocyte migration but the responsible signaling
receptors were not characterized. We report chemotaxis and competitive
binding studies that show LEC binds to and activates CCR1 and CCR8
transfected HEK-293 cells. LEC induced maximal migration of CCR1 and
CCR8 transfected cells at 89.3 nmol/L and cell adhesion at 5.6 nmol/L.
The molar concentration of LEC required to induce maximum cell
migration is 20- to 200-fold greater than that required for RANTES or
I309, respectively. All 3 chemokines induced maximal static adhesion at
5 to 7 nmol/L. A neutralizing polyclonal antibody to LEC was developed
to demonstrate that the unusually high concentration of LEC required to
induce chemotaxis was a property of LEC and not as a result of an
irrelevant protein contamination. This study suggests that LEC may be a
more effective inducer of cell adhesion than cell migration.
(Blood. 2000;96:840-845)
Chemokines are small, usually less than 10 kd, secreted
chemoattractant cytokines.1,2 Chemokines can be divided
into 4 subfamilies, based on a cysteine motif located close to the first 10 to 12 amino acids of the mature protein. The 4 subfamilies are
C, CC, CXC, and CXXXC. The human chemokine LEC (liver-expressed chemokine), a CC chemokine, has a number of different names, including NCC-4, LMC, and HCC-4.3-5 LEC was originally found in an
expressed sequence tag library and later the gene location was
determined to be on human chromosome 17q in the CC chemokine
cluster.3,6 Shoudai et al3 reported 2 sizes of
LEC messenger RNA (mRNA), 1.8 and 0.8 kilobase (kb), both expressed by
unstimulated liver. Hedrick et al5 detected a 0.5-kb
message in most unstimulated lymphoid tissue, but did not detect the
larger message until cells were stimulated with IL-10. These mRNA
species encode a 120 amino acid protein corresponding to a 20 to 24 amino acid propeptide and a 100 amino acid mature protein. Thus, LEC is
an unusually, large CC chemokine with a relatively restricted
expression pattern that makes it difficult to predict its functional role.
Chemokines modulate cell function by interacting with 7 transmembrane
G-protein coupled receptors (GPCRs). Currently, there are at least 9 characterized CC chemokine receptors, CCR1-9.1,7 LEC has been shown to chemoattract both monocytes and lymphocytes but
not neutrophils, which does not indicate what receptor is likely to be
used by LEC.4,5 The maximal chemotactic response to LEC by
either monocytes or lymphocytes was obtained at 89 nmol/L, a
concentration that is 6 to 12 times greater than required for a typical
CC chemokine.1 There is some controversy concerning the
ability of LEC to induce calcium flux in leukocytes or myeloid cell
lines. Youn et al4 did not observe LEC-induced calcium flux, whereas Hedrick et al5 did observe calcium flux in
THP-1 cells. Although both groups used recombinant chemokines, the
proteins differed at their amino termini. To address these concerns, we tested the ability of recombinant LEC to induce calcium flux in human
monocytes. To further characterize LEC and identify a receptor (s), we
performed chemotaxis, adhesion and competitive binding assays with
individual CC receptor transfected HEK-293 cells and found that LEC
uses 2 of the characterized CC receptors.
Reagents and cells
Calcium mobilization
Binding studies Binding assays were performed in triplicate by adding increasing amounts of unlabeled competitor and constant 125I-radiolabeled chemokine, 0.2 ng/assay (RANTES-NEX 292, MIP1 NEX-298, or MIP1 -NEX 299, New England Nuclear, Boston, MA;
I309-IM313, Amersham Pharmacia Biotech, Piscataway, NJ) to individual
1.5-mL microfuge tubes. Two hundred milliliter samples of cells
(5 × 106 cells/mL of monocytes or
2 × 106 cells/mL HEK-transfectants) suspended in
binding media were added to the tubes and mixed by continuous rotation
at room temperature for 45 minutes. After incubation, the cells were
centrifuged through a 10% sucrose/phosphate-buffered saline (PBS)
cushion and the cell-associated radioactivity was measured using a 1272 Wallac gamma counter. A minimum of 2 independent binding assays were
performed in triplicate for each cell type and radiolabeled chemokine.
Scatchard Analysis was performed using LIGAND (Peter Munson, Analytical
Biostatistics section, NIH). The percentage maximal specific binding
was determined in the following manner 1-[(maximum specific
cpm) (competitor cpm)/(maximum specific cpm)] × 100.
Heterologous displacement was performed to provide apparent affinities
for LEC.
Chemotaxis assay Cell migration was assessed using the 48-well microchemotaxis chamber technique. Various chemoattractants, diluted in binding medium (BM) (RPMI 1640 with 1% BSA and 25 mmol/L HEPES), were placed in the lower wells of a chemotaxis chamber. A polycarbonate filter was placed over the chemoattractants; with 5-µm pore size for monocytes and lymphocytes, and 10-µm pore size for HEK-transfectants (Neuroprobe, Cabin John, MD). Membranes were precoated with 10 µg/mL fibronectin or 50 µg/mL rat tail collagen type I (Collaborative Biomedical Products, Bedford, MA) for lymphocytes, THP-1 or transfectants, respectively. A 50-µL cell suspension, 1 × 106 cell/mL for monocytes and transfectants, 5 × 106 cell/mL for lymphocytes, were placed in the upper compartment of the chamber. The chamber was incubated at 37°C (1.5 hours for monocytes, 3 hours for lymphocytes, and 5 hours for transfectants) in a humidified 5% CO2 incubator. At the end of the incubation, the filter was removed, fixed, and stained with Diff-Quik kit (Trends Scientific, Kalamazoo, MI). The migrated cells were counted by computer using the BIOQUANT 95 program (R & M Biometrics, Nashville, TN). The results are expressed as the chemotactic index (average number of cells exposed to chemokine divided by the average number of cells exposed to binding media alone ± SE) migration in triplicate samples and are representatives of at least 3 experiments performed.Adhesion Adhesion assays were adapted from a neutrophil adhesion assay.9 Established human embryonic kidney (HEK)-293 CCR1 or CCR8 transfectants, were suspended at 2 × 106 cells/mL in RPMI-1640 and were labeled with 5 µL of 1 mmol/L calcein AM (Molecular Probes, Eugene, OR) at 37°C for 30 minutes. The 96-well plates were coated with rat tail collagen 0.47 µg/mL, at 37°C for 2 hours, followed by adding adhesion buffer (0.05 mol/L HEPES, 0.15 mol/L NaCl, 1 mmol/L MgCl2, pH 7.4) containing 2% BSA and incubated at room temperature for 1 hour. THP-1 cells were suspended in RMPI-1640 at 5 × 106 cells/mL and loaded with 5 µL of 1 mmol/L calcein AM for 30 minutes at 37°C. The 96-well plates were coated with fibronectin 0.2 µg/mL 100 µL for 2 hours, followed by adding adhesion buffer containing 2% BSA for an additional 1 hour at room temperature incubation. After washing with RPMI-1640, the cells were resuspended in warm RPMI-1640 at the concentration of 1 × 106/mL. Calcein-loaded cell suspension was mixed with 100 µL 2X concentration of LEC, RANTES or chemokine, and anti-LEC and dispensed onto individual wells, followed by 30 minutes incubation at 37°C. Each condition was repeated in triplicate. After careful washing with a multichannel pipettor, the fluorescence of the adherent cells was determined by Cytofluor (PerSeptives Biosytems, Farmingham, MA) using emission wavelength/excitation wavelength 530/485.
We confirmed that LEC is chemotactic and not chemokinetic for human
monocytes, lymphocytes, and THP-1 cells (data not shown). Earlier
studies indicated that LEC could induce calcium flux in a myeloid cell
line, THP-1, and was desensitized by equivalent concentrations of
RANTES.5 To confirm this observation and extend it to a
relevant primary cell system, we determined the ability of LEC to
induce a calcium flux in primary human monocytes. Human monocytes
express high levels of a variety of 7 transmembrane receptors,
including fMLP receptor, CCR1, CCR2 (MCP-1 receptor) CCR5, and CCR8;
therefore, we examined whether the response of monocytes to fMLP,
RANTES, MCP-1, I309 was desensitized by LEC or the reverse. As can be
seen in Figure 1, LEC induced calcium flux
over a broad concentration range. LEC did not reduce MCP-1 or
fMLP-induced calcium flux and interestingly fMLP did not reduce LEC
induced calcium flux (data not shown). I309 did not stimulate calcium
flux in human monocytes. Pretreatment with a 10-fold higher concentration RANTES did reduce LEC-induced calcium flux, similar results were not observed at equivalent concentrations. However, pretreatment of monocytes with LEC from 1 µg/mL to 0.1 µg/mL did reduce RANTES-induced calcium flux. These data suggest that LEC shares
at least one receptor with RANTES and uses another independent of
RANTES.
The chemokines and their receptors are promiscuous and CCR1 seems to
interact with the largest number of ligands. Currently, CCR1 is
documented to be a receptor for RANTES, MIP1 We would like to thank Dr Bob Goldman and his associates at Peprotech
for making LEC and anti-LEC available for study.
Submitted September 15, 1999; accepted March 30, 2000.
Supported in whole or in part with federal funds from the
National Cancer Institute, National Institutes of Health under Contract No NO1-CO-56000.
The content does not necessarily reflect the views or
policies of the Department of Health and Human Services, nor does
mention of trade names, commercial products, or organizations imply
endorsement by the US government.
Reprints: O. M. Zack Howard, PO Box B, Frederick, MD
21702; e-mail: howardz{at}mail.ncifcrf.gov.
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
.001.
MIP1
