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CXC Chemokine Ligand 16 Promotes
Integrin-Mediated Adhesion of
Liver-Infiltrating Lymphocytes to
Cholangiocytes and Hepatocytes within the
Inflamed Human Liver
Mathis Heydtmann, Patricia F. Lalor, J. Albertus Eksteen,
Stefan G. Hübscher, Mike Briskin and David H. Adams
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The Journal of Immunology is published twice each month by
The American Association of Immunologists, Inc.,
1451 Rockville Pike, Suite 650, Rockville, MD 20852
Copyright © 2005 by The American Association of
Immunologists All rights reserved.
Print ISSN: 0022-1767 Online ISSN: 1550-6606.
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J Immunol 2005; 174:1055-1062; ;
doi: 10.4049/jimmunol.174.2.1055
http://www.jimmunol.org/content/174/2/1055
The Journal of Immunology
CXC Chemokine Ligand 16 Promotes Integrin-Mediated
Adhesion of Liver-Infiltrating Lymphocytes to Cholangiocytes
and Hepatocytes within the Inflamed Human Liver1
Mathis Heydtmann,2* Patricia F. Lalor,* J. Albertus Eksteen,* Stefan G. Hübscher,*
Mike Briskin,† and David H. Adams2*
L
ymphocyte trafficking to the liver is important for immunosurveillance, but when it persists unchecked, chronic
inflammation develops, leading to liver damage and eventually fibrosis and cirrhosis. This dichotomy is illustrated by hepatitis C virus (HCV)3 infection. Although T cells must be able to
enter liver tissue to mount a successful immune response against
the virus, these interactions rarely lead to viral clearance, and more
commonly, the virus persists in the presence of continuing chronic
hepatitis and tissue damage (1–3). The mechanisms that regulate
lymphocyte recruitment to, and positioning and persistence within
the liver are poorly understood, but chemokines and their receptors
are likely to play an important role (4).
Lymphocytes first recognize and then adhere to endothelium before extravasating from blood into tissue (5), and it has been suggested that chemokines regulate this process by activating leukocytes
through changes in integrin affinity/avidity (6). This results in firm
*Birmingham University, Edgbaston, United Kingdom; and †Millennium Pharmaceuticals, Cambridge, MA 02139
Received for publication March 23, 2004. Accepted for publication November
2, 2004.
The costs of publication of this article were defrayed in part by the payment of page
charges. This article must therefore be hereby marked advertisement in accordance
with 18 U.S.C. Section 1734 solely to indicate this fact.
1
Funding for this study was provided by The Wellcome Trust (Clinical Training
Fellowship to M.H.) and Digestive Disease Foundation (fellowship to J.A.E.), and
grants from the Wellcome Trust and the European Commission QLG7-CT-199900295.
2
Address correspondence and reprint requests to Drs. Mathis Heydtmann and David H.
Adams, Liver Research Laboratories, Institute of Biomedical Research, Birmingham
University, Edgbaston, B15 2TH, U.K. E-mail addresses: [email protected] and
[email protected]
3
Abbreviations used in this paper: HCV, hepatitis C virus; APAAP, alkaline phosphatase anti-alkaline phosphatase; IMC, isotope-matched control; LIL, liver-infiltrating lymphocyte; PBC, primary biliary cirrhosis; PSC, primary sclerosing cholangitis;
SEC, human sinusoidal endothelial cell; Pa, Pascal.
Copyright © 2005 by The American Association of Immunologists, Inc.
adhesion to the vessel wall and eventual transmigration of the lymphocyte through the endothelium and into the underlying tissue to
sites of infection (7). More than 50 human chemokines have been
identified that bind to and activate ⬎20 different seven-transmembrane-spanning, G protein-linked receptors. Several different chemokine/chemokine receptor interactions may be involved at different
stages of migration from the blood into tissue (8).
CXCL16/CXCR6 is a recently described chemokine/chemokine
receptor pair (9, 10). In human blood, CXCR6 is found on CD8
and CD4 T lymphocytes, NK cells, and NK-T cells (11, 12), and
in mice CXCR6 is detected on CD4, CD8 T cells, and NK cells
within splenic and intraepithelial compartments. Activation of T
cells increases CXCR6 expression (9), which is coordinately regulated with CCR5 and inversely correlated with CXCR4 expression (13). These findings are consistent with reports that CXCR6
is detected predominately on type 1 polarized T cells, including
those in inflamed gut and liver (14, 15). The type 1 immune response that is driven by IL-12 and dominated by IFN-␥ secretion
and cell-mediated immunity is thought to be critical for viral clearance in hepatitis C, and is also implicated in the development of
chronic hepatic inflammation (16, 17). CXCL16 is the only known
ligand of the receptor CXCR6 and is one of only two chemokines,
the other being fractalkine, that exist in a transmembrane as well
as a soluble form (9, 10). CXCL16 mRNA has been detected in
both inflamed and normal liver tissue (9, 14), although the cellular
distribution of CXCL16 protein is not known.
In this study, we show that CXCR6⫹ cells are enriched in normal and chronically inflamed human liver, including chronic hepatitis C-infected liver, and that CXCL16 protein is expressed at
high levels in the liver. Furthermore, CXCL16 on cholangiocytes
was able to promote G protein-dependent, integrin-mediated
adhesion of lymphocytes to VCAM-1 in vitro. These data suggest
0022-1767/05/$02.00
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Lymphocyte recruitment to the liver is critical for viral clearance in acute hepatitis and in the pathogenesis of chronic inflammatory liver disease when persistent chronic inflammation leads to fibrosis and cirrhosis. Chemokines regulate leukocyte recruitment and positioning in tissues and are thus critical regulators of chronic inflammation. The chemokine CXCL16, which is found
in liver tissue, exists in a transmembrane as well as soluble form, providing a potential mechanism for localization to particular
structures. We studied the role of CXCL16 and its receptor CXCR6 in lymphocyte recruitment and retention in the liver. A higher
proportion of CXCR6ⴙ T cells was detected in blood of hepatitis C virus patients compared with healthy subjects, and in chronic
inflammatory liver disease >60% of intrahepatic T cells expressed CXCR6, including CD4, CD8, and CD56ⴙ T cells compared
with <30% in matched blood samples. CXCR6ⴙ lymphocytes were found in association with CXCL16ⴙ bile ducts in portal tracts
and with hepatocytes at sites of interface hepatitis. Analysis of CXCL16 expression and subcellular distribution in cultured human
cholangiocytes, sinusoidal endothelial cells, and hepatocytes revealed that all three cell types expressed CXCL16, with the strongest
staining seen on cholangiocytes. CXCL16 on the cholangiocyte membrane was able to support lymphocyte adhesion by triggering
conformational activation of ␤1 integrins and binding to VCAM-1. Thus, CXCL16 can promote lymphocyte adhesion to epithelial
cells and may function to attract and retain effector cells that promote biliary and hepatocyte destruction in inflammatory liver
disease. The Journal of Immunology, 2005, 174: 1055–1062.
1056
an important role for CXCR6/CXCL16 in the positioning and retention of effector leukocytes in the human liver.
Materials and Methods
Patient characteristics and tissue studied
ml; Sigma-Aldrich), and Tri-iodothyronin (2 nM/ml; Sigma-Aldrich). Adherent cells were used either for immunohistochemical staining or for
adhesion assays. For some experiments, the human cholangiocyte cell line
AKN-1 was used (a kind gift of A. Nussler, Department of General Surgery,
University of Ulm, Ulm, Germany). AKN-1 cells were initially cultured in the
medium described by Nussler et al. (20), and adhesion experiments were compared with AKN-1 cells cultured in our cholangiocyte medium. No differences
were seen in the adhesion results between the two media, and for all subsequent experiments cells were cultured in cholangiocyte culture medium until
confluent on glass coverslips in 48-well plates and used immediately for
adhesion assays.
Isolation of cells
PBL were isolated from venous blood collected into tubes containing
EDTA and diluted 1/1 with PBS. Lymphocytes were isolated by centrifugation at 403 ⫻ g for 30 min at room temperature on a Ficoll (Lymphoprep; Nycomed Pharma) gradient and washed twice with PBS.
LIL were isolated, as described before (18), within 24 h of harvesting.
Liver tissue collected into RPMI 1640 medium (Invitrogen Life Technologies) was diced into 1-mm3 pieces and digested in RPMI 1640 containing
collagenase type 1a (Sigma-Aldrich) at 37°C for 1.5 h. The digested tissue
was passed through a nylon mesh filter (100 ␮m) to remove debris and
washed three times in PBS with FCS (Invitrogen Life Technologies) to
remove collagenase. The cell suspension was layered on a Percoll (Amersham Biosciences) density gradient (30/70%) and centrifuged for 30 min at
717 ⫻ g. The lymphocyte band was removed from the interface between
30 and 70% Percoll, and further washed three times in PBS before resuspension in FCS containing 10% DMSO (Sigma-Aldrich) for storage in
liquid nitrogen using temperature-controlled freezing containers (Nalgene).
Cells were rapidly thawed at 37°C and rested for 2 h before they were used
for adhesion assays or staining for cytometry. Previous experiments comparing fresh lymphocytes with thawed, rested cells showed no difference in
the functional behavior of these cells in a number of different adhesion
assays. It has been previously reported (11) that CXCR6 expression is
modulated by the cell isolation protocol used, and so we investigated the
effect of three different lymphocyte isolation protocols on CXCR6 expression. We compared CXCR6 expression on Ficoll-isolated PBLs, lymphocytes isolated by centrifugation over a Percoll gradient, and cells directly
labeled in whole blood. We did not detect any changes in CXCR6 expression when using these methods. We then incubated PBLs for up to 2 h in
collagenase at the same concentration used in our isolation protocol for
LIL. Again, CXCR6 expression was found to be unchanged. Finally, we
used a nonenzymatic technique described before (18) to isolate lymphocytes from liver tissue, and again detected no effect on CXCR6 expression
compared with the collagenase technique (data not shown).
Human cholangiocytes were isolated according to Joplin (19). The isolation
is similar to the isolation of LIL, with an additional step of positive selection
using magnetic beads (Dynal Biotech) coated with HEA-125 Ab (PROGEN
Biotechnik) after centrifugation over a Percoll density gradient (30/70%). Cells
were cultured until confluent on coverslips (Merck) in cholangiocyte culture
medium consisting of 45% HAM’s F12, 45% DMEM (both from Invitrogen
Life Technologies), and 10% heat-inactivated FCS (Invitrogen Life Technologies) with glutamine (2 mM/ml; Invitrogen Life Technologies), penicillin
(100 U/ml; Britannia Pharmaceuticals), streptomycin (100 ␮g/ml; Celltech
Group), epidermal growth factor (10 ng/ml; Sigma-Aldrich), insulin (0.124
IU/ml; Eli Lilly), hydrocortisone (2 ␮g/ml; Pharmacia), cholera toxin (10 ng/
FIGURE 1. CXCR6⫹ cells are enriched in the liver. A, Percentages of
CXCR6-positive cells in LIL compared with PBL in donors of undiseased
(normal) liver and patients with end-stage chronic HCV. Each point represents a single sample; matched samples from the same donor are linked
with a line. For comparison, values from healthy donors (normal PBL, left
scatter plot) and values for CXCR6 in the blood of HCV⫹ patients without
significant liver disease (HCV PBL) are also shown. B, Percentage of
CXCR6-positive cells in the patients from A, in which matched samples
were available. Values given are mean ⫾ SEM, and p values are given for
statistical comparison between peripheral blood and LIL. C and D, Immunohistochemical expression of CXCR6 in the liver of a normal liver donor
(C) and a patient with end-stage PSC (D). Positive cells stain red with the
APAAP technique (see Materials and Methods). C, In normal liver, occasional CXCR6⫹ lymphoid cells are seen in portal tracts (arrows). D, In
chronic hepatitis associated with PSC, many CXCR6⫹ lymphocytes are
seen infiltrating the portal tracts and some are gathered around bile ducts
(BD). E and F, Histograms of two representative patient samples gated for
Ag-experienced (CD11ahigh) CD8⫹ T cells. PBL are shown in red, and LIL
in black lines and IMC in blue. E, PBL and LIL from a donor of undiseased
liver; F, PBL and LIL from a hepatitis C-infected patient with end-stage
liver disease undergoing liver transplantation. A higher proportion of
CD11ahigh (Ag-experienced) CD8⫹ T cells in the liver expresses CXCR6
compared with the same subset in blood.
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Ethics approval for the study was given by the South Birmingham Local
Research Ethics Committee (Queen Elizabeth Hospital, Birmingham,
U.K.) and the University Hospital Birmingham Trust (Queen Elizabeth
Hospital, Birmingham, U.K.). All liver tissue and peripheral blood were
collected with informed consent. Liver tissue from nondiseased liver and
patients with end-stage hepatitis C cirrhosis as well as primary biliary
cirrhosis (PBC) and primary sclerosing cholangitis (PSC) was used for
immunohistochemical studies (five samples each) and isolation of liverinfiltrating lymphocytes (LIL) (six nondiseased, five HCV, and two PBC
samples). Nondiseased liver was obtained either from patients undergoing
hemi-hepatectomy to remove liver metastases or from organ donors in
which the liver tissue was not used for transplantation. The cases had no
biochemical, virological, or clinical evidence of liver disease, and histology
of the liver showed no significant abnormality. All patients with end-stage
hepatitis C cirrhosis were undergoing transplantation for hepatitis C as the
primary diagnosis and all were HCV-RNA positive by PCR. Diagnosis of
PBC and PSC was made on clinical, immunological, and histological
grounds before orthotopic liver transplantation. Samples of liver tissue (1
cm3) from explanted livers or resected tissue were snap frozen within 1 h
of explantation or resection for later immunohistochemistry. Tissue from
donor organs had been perfused with University of Wisconsin (Madison,
WI) preservation fluid and maintained at 4°C for 12–24 h before being
processed. Matched peripheral blood was obtained from donors of liver
tissue where possible. Peripheral blood was taken at the beginning of the operation before any blood transfusions. Peripheral blood was also collected from
healthy donors and patients with chronic hepatitis C without cirrhosis.
CXCL16 AND CXCR6 IN THE LIVER
The Journal of Immunology
Human sinusoidal endothelial cells (SEC) were isolated using the same
method as for cholangiocytes, but substituting CD31 Ab (10 ␮g/ml; DakoCytomation) during the magnetic bead selection step. Cells were then
cultured in SEC medium containing 10 ng/ml vascular endothelial growth
factor and 10 ng/ml HGF (R&D Systems), as described before (21).
Human hepatocytes were isolated from an encapsulated liver wedge and
cultured overnight in serum-free, arginine-free medium, as described before (22). They were used immediately for immunocytochemistry.
Immunohistochemistry
FIGURE 2. CXCR6 is present on all of the main subtypes of T cells.
CXCR6 is present on the main subtypes of T cells (CD4 and CD8 T cells)
as well as CD56⫹ NK/NK T cells with enrichment in LIL for all subtypes.
A, Each panel shows the percentages of CXCR6⫹ cells in lymphocytes
gated, as indicated on CD3, CD4, CD8, or CD56. LIL are compared with
peripheral blood in normal blood donors (n), donors of undiseased liver
(“n”), and end-stage chronic HCV patients. B, Mean percentages ⫾ SEM
of CXCR6-positive cells in the patients from A, in which matched samples
were available (pooled samples for donors of undiseased liver and HCV
patients). Values of p indicate significance of differences in CXCR6 expression between peripheral blood and LIL.
Western immunoblotting
Protein extracts from liver tissue were blotted on a nitrocellulose membrane (Hybond C-extra; Amersham Biosciences) and incubated overnight
with the primary Ab to CXCL16 (1/250).
Flow cytometry
Up to three-color flow cytometry was conducted on PBL and LIL using
standard techniques (18). Cells were incubated with goat IgG to block Fc
receptors (Sigma-Aldrich; 1 mg/ml), washed with PBS, and then incubated
on ice for 45 min with the IgG2a primary mouse Ab against CXCR6 at
predetermined optimal concentrations (1/500 of clone 7F3; 1/50 clone
7A2) in 100 ␮l of PBS. Cells were washed with cold PBS and further
incubated on ice for 45 min with FITC-conjugated F(ab⬘)2 of goat antimouse Ig (DakoCytomation). Cells were again washed with PBS and incubated with mouse IgG (1 mg/ml; Sigma-Aldrich) to saturate nonspecific
binding sites on the FITC-conjugated F(ab⬘)2. Up to two other Abs (PEconjugated CD8, CD4, CD56 (all from BD Biosciences)); PE-conjugated
CD3 (DakoCytomation); PE-conjugated CD11a, and ECD (PE-Texas
Red)-conjugated CD8, CD3 (from Beckman Coulter) were used in a further
incubation step. After final incubation, cells were washed with PBS and
fixed with 2% paraformaldehyde (Sigma-Aldrich) before analysis in an
Epics XL Coulter flow cytometer (Beckman Coulter) with WinMdi software (The Scripps Research Institute, La Jolla, CA). The lymphocyte population was gated using forward and side scatter parameters to exclude
debris and dead cells, and staining on labeled cells was compared with
staining using matched control Ab. A negative population was gated at
staining intensity of 98% of negative control cells.
Adhesion assays
Cholangiocytes and AKN-1 cells isolated and cultured as described above
were used for the adhesion assays because immunocytochemistry and confocal microscopy had shown the strongest staining of CXCL16 on these
cells (Fig. 4). To investigate the CXCR6/CXCL16 interaction, blocking
Abs were added to lymphocytes (anti-CXCR6, anti-CD18) and/or biliary
cells (anti-CXCL16, anti-VCAM-1) before adhesion. Confluent cell layers
were incubated for 30 min at 37°C in 100 ␮l of the appropriate medium
with anti-CXCL16 (dilutions of a stock solution of 4.33 mg/ml), antiVCAM-1 (1/100, clone BBIG-V1(4B2) from R&D Systems), or isotypematched control Ab, as indicated. A total of 1 ⫻ 105 normal PBLs or LIL
from undiseased liver was incubated with anti-CXCR6 (dilutions of a stock
FIGURE 3. CXCL16 is present in undiseased and chronic HCV-infected
liver. A, Western blot of CXCL16 protein in liver samples from patients transplanted for hepatitis C (HC), alcoholic liver disease (ALD), PBC, or PSC, and
in normal (undiseased) liver (NL). For comparison, samples from spleen and
undiseased colon (normal donors) are also shown. CXCL16 was detected using anti-CXCL16 Abs (1/250) in all liver samples. Actin is shown as a control
for protein loading. B, Mean OD units of five Western blots for each of hepatitis C, normal, PBC, PSC liver (measured by Bio-Rad gel doc), and SEM.
For comparison, mean and SEM for colon and spleen tissue (five samples
each) are also given. Expression in the liver is similar in normal liver compared
with any of the liver diseases. All liver samples have significantly higher
CXCL16 RNA expression than colon or spleen samples, which is highly significant (p ⬍ 0.001 for each comparison).
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Expression of CXCL16 and CXCR6 in liver tissue was studied by immunohistochemistry, as previously described (18). Briefly, sections of snap
frozen liver tissue were fixed in acetone for 10 min, and incubated with
primary mouse anti-human Abs (SD7, anti-CXCL16 IgG1 used 1/10, or
7A2, anti-CXCR6 IgG2a, 1/100) or isotype-matched control for 45 min,
followed by incubation with secondary Ab (rabbit anti-mouse; DakoCytomation). The secondary Ab was detected by indirect alkaline phosphatase
anti-alkaline phosphatase developed with naphtol-AX and fast red
(APAAP) or by an avidin-biotin complex and peroxidase. All incubations
were conducted at room temperature for 45 min, and sections were washed
for 5 min with two changes of TBS, pH 7.4, buffer between incubations.
Endogenous peroxidase activity was blocked using sodium azide (SigmaAldrich). Sections were counterstained with hematoxylin (BDH), and the
staining intensity of CXCL16 and CXCR6 was graded by two observers
(M. Heydtmann and S. Hübscher) using a system previously validated by
confocal microscopy (23). The distribution and intensity of staining in the
following structures were recorded: portal tract, venular and arterial endothelium, biliary epithelium and inflammatory infiltrate, hepatocytes,
Kupffer cells, and sinusoidal and central vein endothelium.
We also assessed the expression of CXCL16 on isolated cholangiocytes,
SEC, and hepatocytes. The cells were cultured overnight on coverslips, fixed
with ethanol for 5 min, and stained as described for tissue sections. Tissue
sections and cultured cells stained using APAAP and fast red were also analyzed using confocal microscopy to determine subcellular localization.
1057
1058
CXCL16 AND CXCR6 IN THE LIVER
T cells, and CD56⫹ cells demonstrated an enrichment of CXCR6
cells within all major subtypes of lymphocytes in the liver (Fig. 2).
Although the percentages are similar between LIL from diseased
and nondiseased liver, absolute numbers of lymphocytes are several
log higher in the HCV livers, and the amount of CXCR6 per cell,
determined by analysis of mean channel fluorescence, was also increased (Fig. 1, D and E). Lymphocytes isolated from the livers of two
patients with PBC were analyzed in the same way, and a similar
enrichment of CXCR6-positive cells was found. Sections of undiseased liver, end-stage hepatitis C-infected liver, and livers from patients with PBC and PSC were stained with anti-CXCR6 Abs. In the
normal liver, CXCR6 staining was generally weak and confined to
occasional leukocytes and dendritic-like cells in portal tracts (Fig.
1C). In contrast, strong staining of CXCR6 was seen in the lymphocyte-rich areas of inflammatory infiltrates in all of the chronic inflammatory liver diseases (Fig. 1D).
Activation of VLA-4 integrin as a result of CXCR6-mediated
intracellular signaling
CXCR6⫹ cells are increased in peripheral blood of patients
with end-stage liver disease due to hepatitis C
To determine whether occupancy of CXCR6 influenced function of the
integrin VLA-4, CXCR6 was engaged using purified rCXCL16 protein
(gift from Millennium Pharmaceuticals). Titration of concentrations between 0.02 and 20 ␮g/ml determined 2 ␮g/ml as the optimum concentration for these assays. VLA-4 activation by manganese (2 mM MnCl; Sigma-Aldrich) was used as a positive control and BSA as a negative control.
To detect changes in VLA-4 activation on mouse and human lymphocytes,
Abs that recognize conformation-dependent epitopes on the activated
integrin were used: 12G10 (24) (IgG1, mouse anti-human; gift from
M. Humphries, School of Biological Sciences, University of Manchester,
Manchester, U.K.) to detect activated human VLA-4 on LIL, and 9EG7
(25) (IgG2a, rat anti-mouse; gift from D. Vestweber, Max Planck Institute
for Immunology, Freiburg, Germany) to detect activated mouse VLA-4 on
L1.2 cells. Incubation with the species-specific primary Ab or isotopematched control (IMC) was performed for 45 min at room temperature and
at the same time as CXCR6 engagement. In some experiments, lymphocytes were preincubated with pertussis toxin (100 ng/ml) for 90 min immediately before addition of ligand to inhibit Gi␣ protein-mediated signaling. In a second step, species-specific FITC-conjugated secondary Ab
(goat anti-mouse or goat anti-rat; Southern Biotechnology Associates) was
used to detect 12G10 or 9EG7, and samples were analyzed by flow cytometry, as described above.
CXCR6 was expressed on 34.7% (⫾6.5) of PBL in end-stage HCV
cirrhosis vs 11.4% (⫾1.6) in normal controls ( p vs cirrhotic patients ⫽ 0.004) and 12.1% (⫾ 3.0) of precirrhotic chronic HCV
patients ( p vs cirrhotic patients ⫽ 0.005). Again, increased percentages of CXCR6⫹ cells were seen in CD3⫹, CD8⫹, CD4⫹, and
CD56⫹ subsets (Fig. 2).
Statistical analysis
For comparison of matched samples, Student’s paired samples t test was
used on the raw numbers where possible, and a probability of ⱕ0.05 (two
tailed) was regarded as significant. For comparison of unpaired results and
means, the nonparametric Mann-Whitney U test was used with the same
significance levels.
Results
CXCR6 expression is increased on LIL
The comparison of CXCR6 levels by flow cytometry on LIL and
matched PBL from organ donors and HCV patients revealed that
more LIL expressed CXCR6 than matched PBL and that levels of
receptor were higher on LIL (Fig. 1). Overall 61.5% of LIL stained
for CXCR6 vs 32.8% of matched PBL (Fig. 1; eight matched samples, p ⫽ 0.004). Increased levels of CXCR6 on LIL were confirmed by analysis of mean channel fluorescence: 18.4 (⫾ 3.8) for
LIL vs 9.7 (⫾ 1.7) for matched PBL. To see whether these differences merely reflect an enrichment of Ag-experienced T cells in
the liver, we compared CXCR6 in blood and liver T cells gated on
CD11ahighCD8⫹. High expression of CD11a discriminates between Ag-experienced and naive CD8 T cells. The levels of
CXCR6 and proportion of CXCR6⫹ cells were higher in the
CD11ahigh LIL than CD11ahigh PBL in both undiseased liver and
HCV, suggesting that CXCR6 is associated with tissue infiltration
(Fig. 1, D and E). Analysis of CD3⫹ T cells, CD8⫹ T cells, CD4⫹
CXCL16 is expressed in normal and chronically inflamed liver
tissue, including chronic hepatitis C-infected liver
We demonstrated the presence of CXCL16 protein in normal,
HCV, and other end-stage cirrhotic livers by Western blotting and
densitometry. CXCL16 was detected in all liver samples studied,
including liver from organ donors and from patients with chronic
inflammatory liver disease. Levels in the liver were much higher
than those detected in other tissues, although densitometry of
Western blots suggested that the total amount of CXCL16 was
similar in nondiseased and diseased liver tissue (Fig. 3). We subsequently used immunohistochemistry to determine the distribution of CXCL16 staining in the chronic inflammatory liver diseases PSC, PBC, and end-stage hepatitis C-infected liver. In
normal liver, CXCL16 was detected on hepatocytes, bile ducts,
and lymphocytes in portal tracts and on sinusoidal cells and occasional cells with a dendritic morphology in the liver parenchyma.
It was absent from portal vessels and central veins (Fig. 4). The
overall staining patterns were similar in the chronic inflammatory
liver diseases, although there was increased staining of sinusoids in
HCV and of bile ducts and ductules in PBC and PSC and increased
focal expression of CXCL16 on periseptal hepatocytes at sites of
interface hepatitis (Table I and Fig. 4, D and E).
CXCL16 is expressed on hepatocytes, cholangiocytes, and
sinusoidal endothelial cells
We investigated subcellular localization of CXCL16 on primary
cultures of different human hepatic cell types. CXCL16 was
strongly expressed on cholangiocytes with moderate expression on
hepatocytes and weak expression on sinusoidal endothelial cells in
culture (Fig. 5). Confocal imaging showed the highest staining
intensity on cholangiocytes, with a membranous pattern, whereas
in hepatocytes staining was overall weaker and strongest in the
cytoplasm (Fig. 5). This led us to use cholangiocytes for the subsequent studies of lymphocyte binding.
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solution of 1.8 mg/ml) or anti-CD18 (1/100) for 30 min at 37°C in 100 ␮l
of PBS. After incubation of the lymphocytes and the cell layers separately,
lymphocytes were added to the biliary cells for a further 30 min of incubation. G protein-mediated signaling was blocked in some assays by adding pertussis toxin (Sigma-Aldrich; 100 ng/ml) to the lymphocytes for 90
min at 37°C before the assay. After incubation, nonadherent lymphocytes
were washed off using PBS, and the cell layers with adherent lymphocytes
were fixed in 70% ethanol. For each experiment, adherent lymphocytes in
at least 10 high power fields of view (surface area of 1 high power field ⫽
0.14 mm2) were counted using a phase contrast microscope. To validate the
method, an initial series of experiments was counted by a blinded investigator (P. Lalor). Flow assays were performed, as described before (21). In
brief, microslides used for lymphocyte perfusion were coated with
VCAM-1 at the concentrations indicated with or without CXCL16 at a
concentration of 10 ␮g/ml for 2 h and were blocked using BSA immediately
before the assay. PBL or LIL was perfused through the microslides at a shear
stress of 0.05 Pascals (Pa), which is comparable to sinusoidal wall shear stress,
and phase contrast video recordings were used to analyze percentage of rolling
and statically adherent cells. Rolling cells moved slowly, but steadily, over the
surface during 5–10 s of observation, while stationary adherent cells did not
make any detectable movement over the same period.
The Journal of Immunology
1059
CXCL16 on cholangiocytes promotes the adhesion of CXCR6⫹
lymphocytes
Having demonstrated high expression of CXCR6 on LIL and
CXCL16 on target cells within the liver, we investigated the ability
of CXCL16 to promote the adhesion of either LIL or PBL to liver
cells using both primary human cholangiocytes and the biliary epi-
thelial cell line AKN-1 (20). These cells were used because of high
staining intensity and membranous expression detected by confocal
immunohistochemistry. A significantly higher proportion of LIL adhered to cholangiocytes compared with PBL (Fig. 6A). Binding of
both PBL and LIL was inhibited by the presence of blocking mAb
against CXCL16 or CXCR6. Lymphocyte adhesion was inhibited by
61 and 47% with anti-CXCL16 and anti-CXCR6, respectively (Fig.
6B). Adhesion blockade was dose dependent, with a maximum effect
Table I. Immunohistochemical staining of CXCL16 in undiseased liver, liver from HCV-infected transplant
patients, and patients transplanted for PBC and PSCa
Portal Fields
Normal
HCV
PBC
PSC
Parenchyma
Bile Duct
Portal
Vessels
Hepatocytes
Sinusoids
Veins
0.5 (0.35)
0.5 (0.5)
0.7 (0.45)**
0.6 (0.55)**
0.1 (0.22)
0.2 (0.3)
0.2 (0.3)
0 (0)
0.4 (0.2)
0.5 (0.5)*
0.5 (0)
0.5 (0)
0.9 (0.2)
2.0 (0)
1.2 (0.45)
1.0 (0)
0
0
0
0
a
Staining was reported by two investigators (M. Heydtmann and S. Hübscher) in portal fields and parenchyma and graded
semiquantitatively according to intensity. 0, No staining seen; 1, weak staining; 2, moderate staining; 3, strong staining, as described
and validated before (23). In addition to endothelial staining of the sinusoids, there were occasional intrasinusoidal cells seen with a
distribution and morphology of Kupffer cells. *, Focal increase at sites of interface hepatitis. **, Focal increase on inflamed bile ducts.
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FIGURE 4. CXCL16 staining in nondiseased and HCV-infected liver.
CXCL16 expression was detected by a peroxidase method in which positive structures are brown (A–C) or an alkaline phosphatase stain (D and E)
in which positive structures stain red. A and B, Nondiseased liver. A, Cytoplasmic staining in a medium-sized bile duct (BD) in a normal portal
tract. B, Staining of sinusoids, including intrasinusoidal monocytic cells
with morphology and distribution of Kupffer cells (arrows). C, HCV-infected liver: diffuse staining of hepatic sinusoidal endothelium. D and E,
CXCL16 staining in chronic hepatitis C stained with an APAAP method
and imaged with light microscopy (D) and confocal microscopy (E). D,
Shows staining of periseptal hepatocytes at an area of bridging fibrosis; E,
shows staining of periseptal hepatocytes (arrows) and vascular endothelium (arrowhead) in a portal tract.
FIGURE 5. CXCL16 is expressed in cholangiocytes, sinusoidal endothelial cells, and hepatocytes. CXCL16 is expressed in cholangiocytes
(left), sinusoidal endothelial cells (center), and hepatocytes (right). Staining was determined using the APAAP technique, with positive staining
showing red. First and second row, Cell lineage-specific positive and negative controls. CK19 is used as a marker of biliary epithelium, CD31 as an
endothelial marker, and CK18 as a lineage specific marker for hepatocytes.
Third row, CXCL16 is detected in all three cell types. Fourth and fifth row,
Confocal microscopy image of CXCL16 stain at higher resolution (single
image sections). Fifth row, The staining intensity of APAAP (red) was
converted into rainbow colors (red ⫽ highest staining intensity; blue ⫽
lowest staining intensity) for comparison. This demonstrates intracellular
staining in all three cell types with a staining pattern particularly suggestive
of membranous staining in cholangiocytes.
1060
CXCL16 AND CXCR6 IN THE LIVER
CXCR6-transfected L1.2 cells were unable to adhere to CXCL16
under static conditions or under low blood flow rates of 0.05 Pa
(data not shown). The experiments were then repeated using immobilized VCAM-1. There was little spontaneous static adhesion
of L1.2 cells to VCAM-1-coated glass slides, but static adhesion of
CXCR6-transfected L1.2 cells to VCAM-1 was activated by the
presence of CXCL16 at 2 ␮g/ml in a time-dependent manner.
Wild-type L1.2 cells lacking CXCR6 did not show CXCL16-mediated adhesion to VCAM-1 (Fig. 7A).
CXCL16 does not activate adhesion to immobilized VCAM-1
under conditions of fluid flow
FIGURE 6. Lymphocyte binding to cholangiocytes is reduced by inhibition of CXCR6/CXCL16. A, LIL show increased adhesion compared with
PBL to cholangiocytes (ⴱ, p ⫽ 0.014). B, Adhesion of both PBL and LIL to
cholangiocytes was reduced using anti-CXCL16 or CXCR6 mAb. In each
experiment, at least 10 high powered fields were counted, and the result was
expressed as percentage of control (addition of an isotype-matched irrelevant
Ab). Lymphocytes were preincubated with anti-CXCR6 Abs or anti-CD18
(blocking adhesion to ICAM), or cholangiocytes were preincubated with antiCXCL16. LIL, five or more experiments each. ⴱ, p ⬍ 0.025 of combined LIL
and PBL experiments vs control experiment without blocking Ab (Student’s t
tests on raw counts). C, Similar levels of adhesion were seen with PBL binding
to primary human cholangiocytes and the cholangiocyte cell line AKN-1. Inhibition of adhesion was conducted as in B using different concentrations of
either anti-CXCL16 or anti-CXCR6.
at a concentration of 45 ␮g/ml CXCL16 or 20 ␮g/ml CXCR6 (Fig.
6C), and no additional effect was gained by combining optimal
concentrations of both Abs (53% inhibition with a mixture of antiCXCR6 and anti-CXCL16). Inhibition of CXCR6/CXCL16 had a
similar effect on adhesion as blockade of CD18 integrin-mediated
binding (58% inhibition), but there was no additive effect when blockade of CXCR6/CXCL16 was combined with anti-CD18 (data not
shown). Incubation of lymphocytes with pertussis toxin inhibited lymphocyte adhesion by 80% (data not shown). Combining anti-CXCR6
or CXCL16 Abs with pertussis toxin did not increase inhibition over
that seen with pertussis toxin alone, implying a major role for G protein-linked signaling.
CXCL16 does not support adhesion in isolation, but triggers
integrin-mediated adhesion to VCAM-1
To determine whether CXCL16 can directly support adhesion, we
conducted static and flow-based adhesion assays using glass microcapillary slides onto which CXCL16 was immobilized.
FIGURE 7. CXCR6 promotes adhesion of lymphocytes to VCAM-1 in
static conditions, but not under conditions of flow. A, Static adhesion:
CXCL16 rapidly triggers static adhesion of CXCR6-transfected L1.2 cells
to VCAM-1. A total of 2 ng/ml CXCL16 was added to L1.2 cells (WT ⫽
wild type; B ⫽ CXCR6 transfectants) on dishes coated with 1 ␮g/ml
VCAM-1 for 0 (control) to 10 min. Manganese chloride was added as a
positive control and induced similar levels of adhesion of wild-type and
CXCR6 transfectants. Only the CXCR6-positive transfectants responded to
CXCL16 with a marked increase in adhesion, which peaked at 2 min. B,
Adhesion of lymphocytes to VCAM-1 under flow. Wild-type and CXCR6transfected L1.2 cells were perfused over VCAM-1 at 0.05 Pa. Adhesion to
VCAM-1 increased with increasing concentration. Coimmobilization of
VCAM-1 and CXCL16 had no additive effect on the number of lymphocytes
binding. Immobilization of CXCL16 in the microslide in the absence of
VCAM-1 was unable to support adhesion of either lymphocyte population.
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To study the role of CXCR6 on adhesion of lymphocytes to immobilized VCAM-1 under flow conditions, we compared adhesion
of L1.2 wild-type and CXCR6-transfected cells with different concentrations of VCAM-1 in the presence or absence of coimmobilized CXCL16. In all experiments, the adhesion of L1.2 cells increased with increasing VCAM-1 concentrations (Fig. 7B). For
CXCR6-transfected L1.2 cells, coimmobilization of CXCL16 and
VCAM-1 did not lead to an increase in lymphocyte adhesion compared with VCAM-1 alone (Fig. 7B). To minimize the possibility
The Journal of Immunology
1061
of competition between CXCL16 and VCAM-1 for immobilization to the glass surface, we coated with either VCAM-1 and
CXCL16 together (Fig. 7B) or in two separate stages (VCAM-1 as
the first step or CXCL16 as first step). There was no difference in
either adhesion of lymphocytes or the amount of immobilized
VCAM-1 bound (detected using Abs) when we examined glass
coated in these different ways (data not shown).
Signaling from CXCR6 leads to activation of the ␣4␤1 integrin
VLA-4
Discussion
Chronic inflammation is characterized by the accumulation of lymphocytes as a consequence of increased recruitment from blood
and retention within the tissue at sites of infection or target cell
damage. Previous studies from our group and others suggest that
specific chemokine/chemokine receptor interactions are involved
in the recruitment of lymphocytes into the liver via either portal or
sinusoidal endothelium, but little is known about the signals that
position and retain lymphocytes at epithelial surfaces within the
liver (18, 26). CXCR6 expression has been reported on activated
extralymphoid lymphocytes, particularly those polarized for Th1
responses (13–15), and we now confirm that CXCR6⫹ cells are
enriched in several major lymphocyte subsets within the liver, suggesting that CXCR6 is associated with liver infiltration. Because
naive T cells are largely excluded from the liver, an alternative
explanation is that the enrichment of CXCR6⫹ cells in the liver is
a consequence of CXCR6 being increased on primed/Ag-experienced T cells compared with naive T cells. To address this, we used
high levels of CD11a expression to discriminate between primed and
naive CD8 T cells and compared expression of CXCR6 on CD8⫹
cells with similarly high levels of CD11a from the liver and blood.
The expression of CXCR6 was markedly higher on primed
(CD11ahigh) CD8 T cells from the liver compared with primed
(CD11ahigh) T cells in blood, suggesting that CXCR6 expression is
associated with tissue infiltration rather than merely reflecting compartmentalization of primed T cells in the liver.
We detected CXCL16 in primary human cholangiocytes and hepatocytes and used cholangiocytes because of their high CXCL16 expression to investigate whether CXCL16 can act directly as an adhe-
FIGURE 8. CXCR6 activates VLA-4 on human and mouse lymphocytes. Activation of VLA-4 on transfected mouse lymphocytes (A and B)
and human LIL (C) by triggering of CXCR6 receptors, as detected with
Abs that recognize activation-dependent epitopes 12G10 (human) and
9EG7 (mouse). A, Titration of VLA-4 response with different concentrations of CXCL16. CXCL16 concentration is plotted against mean channel
fluorescence of 9EG7-staining intensity. Because the response was highest
with a concentration of 2 ␮g/ml, this concentration was used for further
assays. B, Histogram of 9EG7-staining intensity on CXCR6-transfected
L1.2 cells. Compared with IMC shown as gray line, there is staining with
9EG7 on resting L1.2 cells (red). Treatment with manganese (blue) or
CXCL16 (green) leads to a significant increase in 9EG7 staining on the
transfected cells. Preincubation with pertussis toxin (black line) decreases
9EG7 expression to levels comparable with resting cells. C, Histogram of
12G10-staining intensity on human LIL triggered with CXCL16 (green) or
manganese (blue) and control (PBS, red). Treatment with either manganese
or CXCL16 leads to marked increase in 12G10 staining, confirming the
ability of CXCL16 to induce conformational activation of VLA-4.
sion receptor. Direct adhesion has been described to the other
transmembrane chemokine, fractalkine, and more recently to
CXCL16 transfected into COS cells (10, 27, 28). We were able to
demonstrate CXCR6/CXCL16-dependent adhesion of lymphocytes
to human cholangiocytes in vitro, although in contrast to the studies
with COS cells, adhesion to CXCL16⫹ cholangiocytes was inhibited
by pertussis toxin, suggesting that in these human cells signaling via
CXCR6 is required for adhesion rather than a direct adhesive interaction between CXCR6 and CXCL16. There may be several explanations for the differences between our experiments with primary human cells and the transfected COS cells. One obvious difference is the
use of murine lymphocytes with primate epithelial cells in the Shimaoka paper (27). This system does not provide murine VCAM-1 or
ICAM-1 for the murine lymphocytes to bind.
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To demonstrate that occupancy of CXCR6 can activate VLA-4,
leading to increased binding to VCAM-1, we activated CXCR6 on
human LIL and CXCR6-transfected murine L1.2 cells using
rCXCL16. Conformational activation of VLA-4 on human lymphocytes was detected by staining with mAb 12G10, which recognizes an activation-induced epitope on the ␤1 A-domain. Induction of this epitope parallels the activation state of the integrin (24).
The mAb 9EG7, which recognizes an activation-inducible ␤1 neoepitope on murine VLA-4, was used to detect activation on L1.2
cells (25). Incubation of the CXCR6-transfected mouse cell line
L1.2 with CXCL16 led to an increase in the VLA-4 activation
epitope detected by staining with 9EG7 (Fig. 8, A and B). This
peaked at 25 min and was maximal with a concentration of 2
␮g/ml CXCL16 (Fig. 8A). The 9EG7 staining was prevented by
preincubating transfected cells with pertussis toxin (Fig. 8B). The
fact that staining with 9EG7 peaked at only 25 min is consistent
with a conformational activation of the integrin rather than increased protein expression, and suggests a role for CXCR6 in the
activation of lymphocyte adhesion via VLA-4. We next tested the
ability of LIL to respond to CXCL16. A small number of LIL were
12G10 positive in the absence of stimulation, but the majority
expressed 12G10 only after activation with 2 ␮g/ml CXCL16. This
was a similar magnitude response to that seen following treatment
of the cells with manganese (Fig. 8C).
1062
Acknowledgments
We also gratefully acknowledge J. J. Campbell for his helpful comments on
the manuscript and the support from our clinical medical and surgical staff.
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We used functional binding assays and reporter Abs to show
that activation of CXCR6 on LIL triggers ␤1 integrin-mediated
adhesion to VCAM-1. Thus, in vivo CXCL16 could trigger adhesion to VCAM-1, which is strongly expressed on inflamed bile
ducts (29). To investigate the mechanism of CXCL16-mediated
adhesion, we activated either L1.2 CXCR6⫹ transfectants or
CXCR6high LIL with CXCL16 and studied activation of VLA-4.
Occupancy of CXCR6 by ligand resulted in the detection of activation-dependent epitopes on VLA-4, confirming that CXCL16
can induce conformational activation of lymphocyte integrins.
However, immobilized rCXCL16 had no effect on lymphocyte adhesion in flow-based adhesion assays, and this together with the
higher levels of CXCL16 detected on epithelial cells compared
with vascular endothelium suggests that CXCR6/CXCL16 interactions may be more important for maintaining stable adhesion to
epithelial cells. CXCR6-expressing murine NK-T cells fail to migrate to soluble CXCL16 (30), and it has been postulated that
membranous CXCL16 may be required for direct cell-cell adhesion and the facilitation of migration on or through epithelium or
endothelium. Our data suggest that adhesion of effector lymphocytes to cholangiocytes will require not only CXCL16 expression,
but also the presence of VCAM-1 to support integrin-mediated
adhesion. Thus, the lack of VCAM-1 on nondiseased bile ducts
might prevent the development of bile duct damage even in the
presence of constitutive CXCL16 expression.
The fact that many of the lymphocytes isolated from the livers
of organ donors were CXCR6high suggests that CXCR6/CXCL16
interactions may be involved in the positioning and retention of
lymphocytes in normal liver. Normal liver contains a large number
of conventional T cells, which include a population of CD8 T cells
closely associated with bile ducts (31) as well as NK and NK T
cells (32, 33). The high levels of CXCR6 expressed by NK T cells
and some other effector cells in blood may be an important factor
in the recruitment and retention of these cells within the liver. The
normal livers we studied were obtained from organ donors, and we
cannot exclude the possibility that T cells are recruited to these
livers as part of a low grade inflammatory response (34). However,
there was no biochemical or histological evidence of pathological
inflammation in any of the normal specimens.
In summary, we propose an important role for CXCL16 in the
recruitment and retention of CXCR6⫹ effector cells in the human
liver during inflammatory liver disease, and suggest that this chemokine/receptor pair is a potential therapeutic target to prevent
inflammatory damage in chronic hepatitis.
CXCL16 AND CXCR6 IN THE LIVER