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Multiple Chemokine Receptors, Including
CCR6 and CXCR3, Regulate
Antigen-Induced T Cell Homing to the
Human Asthmatic Airway
Seddon Y. Thomas, Aleena Banerji, Benjamin D. Medoff,
Craig M. Lilly and Andrew D. Luster
J Immunol 2007; 179:1901-1912; ;
doi: 10.4049/jimmunol.179.3.1901
http://www.jimmunol.org/content/179/3/1901
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Copyright © 2007 by The American Association of
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References
The Journal of Immunology
Multiple Chemokine Receptors, Including CCR6 and CXCR3,
Regulate Antigen-Induced T Cell Homing to the Human
Asthmatic Airway1
Seddon Y. Thomas,* Aleena Banerji,* Benjamin D. Medoff,*† Craig M. Lilly,‡
and Andrew D. Luster2*
H
uman allergic asthma is a chronic inflammatory disease
characterized by airway eosinophilia, production of allergen specific-IgE, Th2 cytokine production, mucus hypersecretion, airway hyperresponsiveness, and airway remodeling (1, 2).
T lymphocytes play an important role in promoting the asthmatic
response through the production of Th2 cytokines, such as IL-4, IL-5,
and IL-13. Recent data also suggest that a specific subset of T cells,
CD1d-restricted invariant NKT cells, may play a significant role in the
asthmatic response and make up ⬎60% of T cells isolated from bronchoalveolar lavage (BAL)3 fluid (3). In addition, regulatory T cells
have been shown to suppress an overexuberant asthmatic response
(4), and Th1 lymphocytes have been shown to be capable of both
increasing or decreasing the severity of the asthmatic response (5, 6).
Because T lymphocytes play critical roles in promoting and modulating the asthmatic response, it is important to study the mechanism
of T cell recruitment into the human asthmatic airway.
*Center for Immunology and Inflammatory Diseases, Division of Rheumatology, Allergy and Immunology, Massachusetts General Hospital and Harvard Medical School,
Charlestown, MA 02129; †Pulmonary and Critical Care Unit, Massachusetts General
Hospital and Harvard Medical School, Boston, MA 02114; and ‡Department of Medicine, University of Massachusetts Medical School, Worcester, MA 01655
Received for publication February 9, 2007. Accepted for publication May 22, 2007.
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
This work was supported by National Institutes of Health Grants R01 AI40618 and
T32 AI060548 and the Dana Foundation grant for Human Immunology.
2
Address correspondence and reprint requests to Dr. Andrew D. Luster, Center for
Immunology and Inflammatory Diseases, Division of Rheumatology, Allergy and
Immunology, Massachusetts General Hospital, Building 149-8301, 13th Street,
Charlestown, MA 02129. E-mail address: [email protected]
3
Abbreviations used in this paper: BAL, bronchoalveolar lavage; PB, peripheral
blood; CBA, cytometric bead array; MFI, mean fluorescence intensity; FEV1, forced
expiratory volume in 1 s; FVC, forced vital capacity.
Copyright © 2007 by The American Association of Immunologists, Inc. 0022-1767/07/$2.00
www.jimmunol.org
Homeostatic and tissue-specific trafficking of T cells is required
for effective immune surveillance. T lymphocytes are recruited to
tissue- and inflammation-specific sites through the expression of
specific chemoattractant receptors and encounter with cognate
lipid or peptide ligands. Certain chemokine receptors have been
associated with T cell homing to tissue-specific sites, including
CCR7 and CXCR5 for lymph node, CCR4 and CCR10 for skin,
and CCR9 for small intestine (7). No chemoattractant receptor has
been specifically linked with homing to the lung or air spaces.
In addition to homeostatic and tissue-specific trafficking at baseline, T lymphocytes must respond to and be recruited into sites of
Th1 or Th2 inflammation. With Th1-type inflammation, production of STAT1-inducible chemokines leads to recruitment of Th1
and effector CD8 T cells through the cognate Th1-associated
chemokine receptors, CCR5, CXCR3, and CXCR6 (8). However, with Th2-type inflammation, production of STAT6-inducible chemokines leads to recruitment of Th2 cells through the
cognate Th2-associated chemokine receptors, CCR3, CCR4,
and CCR8 (9). Although these Th1- or Th2-associated receptors
have been observed on polarized T cells in vitro, the chemoattractant receptor expression pattern on Th1 or Th2 cells ex vivo
is more complex.
To study human allergic asthma and the in vivo recruitment of
T cells into the allergic airway, we have used a segmental allergen
challenge protocol. Segmental allergen challenge allows pre- and
postallergen challenge comparison of BAL T cells and other leukocytes within the same subject and mimics the human acute asthmatic response in a controlled setting. Each subject serves as its
own control, providing specific information about the in vivo asthmatic response. The asthmatic response can be divided into an
early and a late phase. The early phase (5– 60 min) is typified by
airway swelling and smooth muscle cell constriction and results from
mast cell degranulation. The late phase (⬎4 h) is typified by lymphocyte and eosinophil recruitment to the airway (10). Because we were
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Human allergic asthma is a chronic inflammatory disease of the airways thought to be driven by allergen-specific Th2 cells, which
are recruited into the lung in response to inhaled allergen. To identify chemoattractant receptors that control this homing pattern,
we used endobronchial segmental allergen challenge in human atopic asthmatics to define the pattern of chemoattractant receptor
expression on recruited T cells as well as the numbers of recruited CD1d-restricted NKT cells and levels of chemokines in the
bronchoalveolar (BAL) fluid. CD1d-restricted NKT cells comprised only a small minority of BAL T cells before or after Ag
challenge. BAL T cells were enriched in their expression of specific chemoattractant receptors compared with peripheral blood T
cells prechallenge, including CCR5, CCR6, CXCR3, CXCR4, and BLT1. Surprisingly, following segmental allergen challenge, no
chemoattractant receptor was specifically increased. However, CCR6 and CXCR3, which were expressed on virtually all CD4ⴙ
BAL T cells prechallenge, were markedly decreased on all recruited BAL T cells following Ag challenge, suggesting that these
receptors were internalized following encounter with ligand in the airway. Our data therefore suggests a role for CCR6 and
CXCR3, in conjunction with other chemoattractant receptors, in the recruitment of inflammatory T cells into the BAL during the
allergic asthmatic response. The Journal of Immunology, 2007, 179: 1901–1912.
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CHEMOKINE RECEPTORS ON HUMAN ASTHMATIC AIRWAY T CELLS
Table I. Asthmatic subject characteristics, lung function tests, total serum IgE, and allergen dose used in segmental allergen challengea
FEV1
Subject
Symbol
Gender
Age
Race
Percentage of
Predicted
FEV1:FVC
Total IgE
Allergen
Challenge Dose
1
2
3
4
5
䡺
{, …
„, ⫹
⫻
ⴱ, 䡬
F
F
M
F
M
46
27
48
64
27
African American
Caucasian
African American
Caucasian
Caucasian
78.8
85.6
83.4
89.9
88.9
0.66
0.79
0.72
0.83
0.72
204
158
331
220
256
C
DP
C
C
C
0.7
185, 20
20, 20
69
2.2, 20
a
Symbols that represent a subject are listed here and are used throughout the article for total serum IgE are kilounits per liter. Units for allergen dose are measured either
in bioequivalency allergy units per milliliter for cat hair allergen or in arbitrary units per milliliter for D. pteronyssinus allergen. Allergen dose in segmental allergen challenge
was based on responsiveness to skin testing. In some instances, allergen challenge was performed on the same subject at a separate time and is indicated by a different symbol
for the same subject. C, Cat hair; DP, D. pteronyssinus.
Materials and Methods
Segmental allergen challenge
Each subject provided written informed consent using forms approved by the
Partners Healthcare Institutional Review Board. All subjects met the American
Thoracic Society’s definition of asthma (11), had disease of mild severity
based on spirometry and physician assessment (12), and had symptoms to cat
or dust mite exposure with a corresponding positive skin prick test. Subjects
were selected on a volunteer basis. Although some subjects had a history of
inhaled corticosteroid use, subjects were not on corticosteroids for 1 mo before
the study. Subjects were on no other medications except short-acting ␤-agonists for asthma and loratidine for nasal symptoms, which were withheld 12 h
before the bronchoscopy. The dosage of standardized allergen for bronchoscopic challenge was determined from quantitative skin testing (13). Segmental allergen challenge was performed at least 4 wk after measurements of atopy
and any symptoms of infection as previously described (13). Briefly, bronchoscopy was performed under conscious sedation with a total of ⬍400 mg of
topical lidocaine. The bronchoscope was advanced to airway occlusion in the
anterior segment of the left upper lobe, three 50-ml aliquots of warmed sterile
saline were serially instilled, and prechallenge BAL fluid was recovered into
Teflon containers by gentle aspiration. The bronchoscope was then moved to
the right middle lobe, where 1 ml of standardized allergen solution (cat or dust
mite) was delivered. The bronchoscope was then removed, and focal wheezing
was confirmed to be present exclusively over the right middle lobe in all
subjects by auscultation. Twenty-four hours later, Ag challenge BAL fluid was
obtained from the right middle lobe site. PB was drawn at both the prechallenge and postchallenge time points.
Allergen extract
Standardized allergen extract for cat hair and Dermatophagoides pteronyssinus were purchased from Greer Laboratories. Standardized cat hair
allergen extract contained ⬍1 ng/ml endotoxin; standardized D. pteronyssinus allergen extract contained 9 ng/ml endotoxin.
Cytospin
Cell differential counts for prechallenge and postchallenge BAL were determined by enumerating alveolar macrophages, neutrophils, eosinophils,
and lymphocytes on cytocentrifuge preparations stained with a combination of Wright stain (EM Sciences) and Diff-Quick (Dade Behring).
Flow cytometry reagents
Abs to CCR1 (53504.111), CXCR1 (42705.111), CCR2 (48607.121),
CXCR2 (48311.211), CCR3 (61828.111), CXCR5 (51505.111), CXCR6
(56811), CCR7 (150503), CCR9 (112509) were purchased from R&D Systems. CXCR3 (1C6), CCR4 (1G1), CXCR4 (12G5), CCR5 (3A9), CCR6
(11A9), CCR7 (2H4), CD3 (UCHT1), CD4 (SK3), CD8␣ (RPA-T8),
CD19 (SJ25C1), CD25 (M-A251), CD27 (M-T271), CD45RA (HI100),
CD62L (Dreg 56), IFN-␥ (B27), and IL-4 (MP4 –25D2) were purchased
from BD Pharmingen. V␣24 (C15) was purchased from Beckman Coulter.
CX3CR1 (2A9-1) was purchased from MBL. BLT1 (202/7B1) was purchased
from Serotec. Abs used in these experiments were directly conjugated to their
respective fluorochromes except for CXCR6 in which a primary Ab was used
in combination with a fluorochrome-conjugated secondary Ab.
6B11 mAb is directed against an invariant V␣24J␣Q epitope possessed
by NKT cells. Dual staining with V␣24 and 6B11 enables specific identification of a canonical TCR rearrangement on NKT cells, comparable in
specificity to tetramer staining.
Flow cytometry staining
For extracellular epitopes, BAL and whole PB were blocked with 10%
human serum and stained in PBS with 1% FCS. Whole PB was lysed
following staining with FACS Lysing Solution (BD Biosciences). Cells
were then fixed with 2% paraformaldehyde.
For intracellular cytokine staining, BAL and PB were incubated in RPMI
1640 with 10% FCS in the absence of exogenous stimulation or in the presence
of PMA and ionomycin. After 1 h, Golgiplug (BD Pharmingen) was added to
block cytokine secretion, and cells were incubated for an additional 5 h before
staining for extracellular epitopes (CD4 and CD8). Cells were then fixed and
permeabilized with Fix & Perm (Caltag Laboratories) and then stained for
intracellular IFN-␥ and IL-4.
To determine total chemokine receptor levels (both extracellular and
intracellular), BAL and PB were stained with CD3, CD4, and CD8 as
described above, fixed, and permeabilized with Fix & Perm (Caltag Laboratories) and then stained for the chemokine receptor of interest.
Samples were run on a FACSCalibur (BD Biosciences) cytometer and
analyzed with either CellQuest or FlowJo. BAL and PB lymphocytes were
specifically analyzed using forward and side scatter properties as previously described (14).
Cytometric bead array (CBA) and ELISA
Chemokines were measured by CBA or ELISA using either neat or
10-fold concentrated BAL supernatant. BAL was concentrated in Centriplus
YM-3 centrifugal filter devices (Millipore). Levels of CXCL8, CXCL9,
CXCL10, CCL2, and CCL5 in prechallenge and postchallenge BAL fluid
were measured with the human chemokine CBA (BD Pharmingen) using a
FACSCalibur cytometer. Levels of CXCL11, CXCL16, CCL11, CCL17,
CCL20, CCL22, and CCL26 were determined by ELISA (R&D Systems).
Magnetic bead separation of CD4 T cells from BAL and PB
PBMC were prepared by centrifugation through a density gradient on Histopaque-1077 (Sigma-Aldrich). To select for CD4 T cells, BAL cells and
PBMC were initially depleted of monocytes by negative selection with
anti-CD14 magnetic beads according to the manufacturer’s protocol
(Miltenyi Biotec). The CD14-depleted BAL cells and PBMC were then
positively selected with anti-CD4 magnetic beads. Purity was evaluated by
quantitative PCR with primers for CD4, CD8, CD19, and CD14 to determine
the contribution of unwanted cell subsets. Magnetically selected CD4 T cells
from BAL were ⬎92% pure and from PB were ⬎96% pure (data not shown).
Quantitative PCR
Quantitative PCR was performed on cDNA obtained from total RNA extracted from magnetically isolated CD4 T cells as previously described.
Primers are published online at www.immunologynet.org.
Internalization
BAL or PB cells were placed in RPMI 1640 with 10% FCS at a concentration of 1 million cells/ml and allowed to equilibrate to 37°C in the
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interested in T lymphocyte recruitment following challenge, we characterized the percentage of CD1d-restricted NKT cells, chemoattractant receptor profile, cytokine, and memory phenotype of peripheral
blood (PB) and BAL T cells, and production of chemoattractant ligands before and 24 h after segmental allergen challenge.
The Journal of Immunology
1903
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FIGURE 1. Chemoattractant receptor expression is increased on CD4⫹ and CD8⫹ BAL T cells of asthmatic subjects as compared with PB T cells
at baseline. A, Flow cytometry staining for chemoattractant receptor expression (CD4 or CD8 on x-axis and chemoattractant receptor on y-axis) is
shown for a representative asthmatic subject (square symbol) for CD4⫹ and CD8⫹ PB and BAL T cells. B, The percentage of CD4⫹ or CD8⫹ PB
or BAL T cells that express a specific chemokine receptor at baseline is displayed. C, The MFI for chemoattractant receptors on CD4⫹ or CD8⫹
PB or BAL T cells at baseline is displayed. D, Copies of chemoattractant receptor per copy of GAPDH is shown for cDNA isolated from CD4⫹
PB or BAL T cells at baseline. Each symbol represents an individual subject with the black bar representing the mean (as shown in Table I).
incubator for 30 min. In each tube, various concentrations of chemokine (or
no chemokine control) were then added to each well and cells were allowed
to incubate for 30 min. After this time, each well was divided in two for
staining for either extracellular or total (both extracellular and intracellular)
chemokine receptor expression. Cells were stained at 4°C to prevent further
internalization or re-expression of the chemokine receptor of interest.
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CHEMOKINE RECEPTORS ON HUMAN ASTHMATIC AIRWAY T CELLS
FIGURE 2. Lymphocytes and eosinophils accumulate in the BAL following segmental allergen challenge.
A, Baseline and allergen challenge BAL total, lymphocytes, eosinophils, alveolar macrophages, and polymorphonuclear neutrophil (PMN) cell numbers. Each symbol represents an individual subject with the black bar
representing the mean (as shown in Table I). B, Percentage of lymphocytes, eosinophils, alveolar macrophages, and polymorphonuclear neutrophils from baseline and allergen challenge BAL segments based on
cytospin counts from five subjects.
Samples were analyzed for statistically significant differences using the
two-tailed paired Student t test with p ⬍ 0.05 considered statistically
significant.
Results
Selection of allergic asthmatic subjects for segmental allergen
challenge study
Asthmatic subjects were selected with known allergy to cat or dust
mite (Table I). Lung function tests were performed on each subject
to determine their percent of predicted forced expiratory volume in
1 s (FEV1) and FEV1:forced vital capacity (FVC) ratio, and total
serum IgE levels were measured. Values were consistent with mild
to moderate obstructive airway disease and a clinical diagnosis of
asthma. Each subject reacted to allergen exposure with visible airway narrowing and focal wheezing exclusively over the challenged lung segment. Each subject served as their own control
because comparisons were made between paired PB and BAL or
paired pre- and postchallenge BAL.
quantitative PCR because Abs to these receptors were not commercially available. CCR8 was found at similar levels in CD4⫹ PB
and BAL T cells, while CCR10 was significantly decreased in
CD4⫹ BAL T cells as compared with PB (Fig. 1D). In addition,
although CCR3, CCR4, CCR5, CCR7, CXCR5, and CXCR6 reflected a similar pattern of RNA levels and surface chemoattractant
receptor expression in CD4⫹ PB and BAL T cells, the RNA levels
of CCR6, CXCR4, and BLT1 were unchanged, variable, or even
the opposite of what was observed for surface receptor expression.
This suggests that the surface expression of specific receptors may
be regulated at translational or posttranslational steps and that
measuring RNA levels may not always provide an accurate reflection of surface expression for all chemoattractant receptors.
Chemoattractant expression profile on PB and BAL T cells at
baseline in asthmatic subjects
Initially, we examined the surface chemoattractant receptor profile
on CD4⫹ and CD8⫹ PB and BAL T cells at baseline by flow
cytometry (Fig. 1, A–C). We hypothesized that specific chemoattractant receptors would be important for homing to the airway at
baseline and observed the percentage of CCR1, CCR5, CCR6,
CCR9, CXCR1, CXCR2, CXCR3, CXCR4, CXCR6, and BLT1
were significantly enriched on CD4⫹ BAL T cells as compared
with CD4⫹ PB T cells. A smaller subset of these receptors, including CCR5, CCR6, and BLT1 were significantly enriched as a
percentage on CD8⫹ BAL T cells as compared with CD8⫹ PB T
cells (Fig. 1B). In addition, we also examined the mean fluorescence intensity (MFI), a measure of receptor density per cell. We
found that the MFI for CXCR3, CXCR4, CCR5, and CCR6 was
significantly increased on both CD4⫹ and CD8⫹ BAL T cells as
compared with PB T cells (Fig. 1C).
To study receptor expression when mAbs were not available and
to determine whether differences observed in surface chemoattractant receptor expression were reproduced at the RNA level, we
isolated RNA from CD4⫹ PB and BAL T cells and used quantitative RT-PCR to compare the copies of each receptor per copy of
GAPDH (Fig. 1D). CCR8 and CCR10 were only examined by
FIGURE 3. NKT cells are enriched in BAL as compared with PB but
are not the predominant lymphocyte population in the BAL. A, Flow cytometry staining for NKT cells (V␣24⫹ 6B11⫹) is shown for a representative asthmatic subject (square symbol) from PB and BAL before allergen
challenge and BAL following segmental allergen challenge at 24 h. B, The
percentage of NKT cells in the lymphocyte gate is shown for each subject
for prechallenge PB and pre- and postchallenge BAL. Each symbol represents an individual subject with the black bar representing the mean (as
shown in Table I).
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Statistics
The Journal of Immunology
1905
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FIGURE 4. Chemoattractant receptor expression is decreased for CCR6 and CXCR3 on CD4⫹ and CD8⫹ BAL T cells following segmental allergen
challenge. A, Flow cytometry staining for chemoattractant receptor expression (CD4 or CD8 on x-axis and chemoattractant receptor on y-axis) is shown
for a representative asthmatic subject (square symbol) for CD4⫹ and CD8⫹ BAL T cells before and 24 h following segmental allergen challenge. B, The
percentage of CD4⫹ or CD8⫹ BAL T cells that express a specific chemokine receptor before and after allergen challenge is displayed. C, The MFI for
chemoattractant receptors on CD4⫹ or CD8⫹ BAL T cells before and after allergen challenge is displayed. D, Copies of chemoattractant receptor per copy
of GAPDH is shown for cDNA isolated from CD4⫹ BAL T cells before and 24 h following segmental allergen challenge. Each symbol represents an
individual subject with the black bar representing the mean (as shown in Table I).
Cellular recruitment into BAL following segmental allergen
challenge
To observe the recruitment of cells into the human asthmatic airway in vivo, we used a segmental allergen challenge protocol. We
tested the skin allergen responsiveness of each subject and used
this to determine the allergen dose for segmental allergen chal-
lenge. At baseline, prechallenge BAL was procured from the left
upper lobe by bronchoscopy and then allergen instilled in the right
middle lobe of the lung. After 24 h, postchallenge BAL was taken
from the challenged lung segment. PB was drawn at baseline and
at 24 h following segmental allergen challenge. Pre- and postchallenge PB T cells were similar in terms of NKT cell populations,
1906
CHEMOKINE RECEPTORS ON HUMAN ASTHMATIC AIRWAY T CELLS
chemokine receptor expression profiles, intracellular cytokine
staining, and memory markers, demonstrating that the segmental
allergen challenge induced tissue-specific but not systemic T cell
responses to allergen challenge (data not shown).
To compare the recruitment of cells to the BAL pre- and postchallenge, the total number of cells recovered was enumerated and
differential cell counts determined by cytospin (Fig. 2A). The total
number of cells recruited into the BAL varied from subject to
subject but on average increased ⬎7-fold from baseline. In terms
of differential cell counts, lymphocytes increased an average of
⬎15-fold, eosinophils increased ⬎250-fold, and alveolar macrophages increased only ⬃3-fold. Neutrophils increased ⬎80-fold on
average but were not consistently increased as shown by the distribution on the graph. The percentage of lymphocytes and eosinophils in the BAL increased significantly following allergen challenge indicative of an allergic response, while the percentage of
alveolar macrophages decreased significantly following challenge
(Fig. 2B).
NKT cells are enriched in BAL as compared with PB but are
not the predominant lymphocyte in asthmatic lung
A recent report suggested that NKT cells account for ⬎60% of T cells
in the BAL from asthmatic subjects but not sarcoid or healthy controls
(3). Because Ag-specific Th2 cells have been thought to be the predominant lymphocyte that promotes the asthmatic response, we examined PB and BAL from asthmatic subjects for the presence of NKT
cells before and after segmental allergen challenge. CD1d-restricted
NKT cells can be identified based on either staining with CD1d tetramer loaded with a surrogate ligand for NKT cells, ␣-GalCer, or by
double staining with the Abs, 6B11, and V␣24. 6B11 recognizes the
invariant V␣24J␣Q rearrangement on the TCR V␣24 chain, but 6B11
staining in the absence of staining for the V␣24 chain may actually
include B or non-CD1d-restricted T cells. Staining with CD1d tetramer loaded with ␣-GalCer or double staining with 6B11 and V␣24
Abs has been shown to recognize similar numbers of CD1d-restricted
NKT cells from human PB (15).
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FIGURE 5. BAL T cells are skewed toward a Th2 response in the absence of ex vivo stimulation but are capable of producing IFN-␥ when stimulated,
and postallergen challenge BAL T cells have memory characteristics more similar to prechallenge PB than prechallenge BAL T cells. A, Intracellular
cytokine staining for IFN-␥ and IL-4 from CD4⫹ and CD8⫹ T cells (CD4 or CD8 on x-axis and IFN-␥ or IL-4 on y-axis) in the absence of stimulation
(⫺) and following treatment with PMA and ionomycin (⫹) from a representative subject (square symbol). B and C, The percentage of PB or BAL CD4⫹
or CD8⫹ T cells before and 24 h following segmental allergen challenge producing IFN-␥ or IL-4 in the absence of stimulation (B) or following treatment
with PMA and ionomycin (C). Each symbol represents an individual subject with the black bar representing the mean (as shown in Table I). D and E, Flow
cytometry staining for memory phenotype (CCR7 on x-axis and CD45RA on y-axis) for PB or BAL CD4⫹ (D) or CD8⫹ T cells (E) before and 24 h
following segmental allergen challenge from a representative asthmatic subject (square symbol). F and G, The percentage of PB or BAL CD4⫹ (F) or CD8⫹
T cells (G) before and 24 h following segmental allergen challenge that express each memory phenotype as indicated: naive (CD45RA⫹CCR7⫹), CCR7⫹
memory (CD45RA⫺CCR7⫹), CCR7⫺ memory (CD45RA⫺CCR7⫺), and RA-re-expressing CCR7⫺ memory (CD45RA⫹CCR7⫺, CD8 only). Each symbol
represents an individual subject with the black bar representing the mean (as shown in Table I).
The Journal of Immunology
1907
In this study, we identified CD1d-restricted NKT cells through
costaining with 6B11 and V␣24 Abs (Fig. 3). CD1d-restricted
NKT cells were found at low levels in prechallenge PB (0.0099 –
0.26% of lymphocyte gate) but were significantly increased in prechallenge BAL (0.39 –2.16%) from the asthmatic subjects, as previously described (14). Interestingly, the percentage of BAL
CD1d-restricted NKT cells following segmental allergen challenge
was similar to levels found in prechallenge BAL. This suggests
that CD1d-restricted NKT cells were recruited into the asthmatic
lung following segmental allergen challenge as part of an increase
in total lymphocytes but were not preferentially recruited in comparison to other lymphocyte subsets. These data also demonstrate
that NKT cells are not the major CD4⫹ T lymphocyte in the
asthmatic BAL.
Chemoattractant receptor expression profiles from BAL T cells
before and after segmental allergen challenge
To determine the significance of specific chemoattractant receptors
in recruitment of T cells to the asthmatic lung, we examined the
chemoattractant expression profile for CD4⫹ and CD8⫹ BAL T
cells before and 24 h following segmental allergen challenge
(Fig. 4, A–C). Although we predicted that we would see an
increase in Th2-associated chemoattractant receptor expression
(CCR3, CCR4, CCR8) on BAL T cells following segmental allergen challenge, no receptor was significantly increased in comparison to prechallenge BAL T cells as a percentage or by MFI (Fig.
4, B and C). Surprisingly, we found that CCR6 and CXCR3 were
significantly decreased both as a percentage and as mean fluorescence intensity on CD4⫹ and CD8⫹ BAL T cells and that CXCR5
was significantly decreased as a percentage on CD4⫹ BAL T cells
following segmental allergen challenge (Fig. 4, B and C).
Although the MFI for CCR7 on CD8⫹ BAL T cells was significantly decreased following challenge, CCR7 was increased on
CD8⫹ BAL T cells on a percentage basis (Fig. 4, B and C). This
trend was also true for CD4⫹ BAL T cells, although the findings
do not reach statistical significance. We would suggest that the
higher percentage of T cells expressing CCR7 implies that a higher
percentage of T cells have lymph node homing potential.
We also compared the total number of chemoattractant receptorpositive CD4⫹ and CD8⫹ BAL T cells before and after segmental
allergen challenge and found that the number of CD4⫹ or CD8⫹
T cells expressing each chemoattractant receptor examined was
increased except for CXCR5⫹ CD4⫹ T cells, which were found at
lower levels postchallenge (data not shown). In addition, RNA
levels of CCR8 or CCR10 in CD4⫹ BAL T cells were unchanged
following segmental allergen challenge (Fig. 4D).
To examine whether the decrease in chemoattractant receptor
expression was regulated at the RNA level or reflected a posttranscriptional alteration in surface expression, we isolated RNA from
CD4⫹ BAL T cells before and 24 h following segmental allergen
challenge (Fig. 4D). There were no statistically significant changes
in RNA of any chemoattractant receptor. Although CCR6 and
CXCR5 surface protein levels were significantly decreased following segmental allergen challenge, CCR6 and CXCR5 RNA levels
were similar pre- and postchallenge. This suggests that the decrease in CCR6 and CXCR5 surface expression was regulated
posttranscriptionally.
BAL T cells from asthmatic subjects are skewed toward IL-4
production in the absence of exogenous stimulation but retain
ability to produce IFN-␥
Because specific chemoattractant receptors have been associated
with Th1 or Th2 cytokine production, we determined the composition of IFN-␥ and IL-4 producing CD4⫹ and CD8⫹ T cells in the
PB and BAL pre- and postchallenge (Fig. 5, A–C). In the absence
of exogenous stimulation, we found that the percentage of IL-4producing CD4⫹ BAL T cells was higher than the percentage of
IFN-␥-producing CD4⫹ BAL T cells (Fig. 5B). However, the
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FIGURE 6. Specific chemokines (including CCR6 and CXCR3 ligands) are increased in the BAL following segmental allergen challenge. The graph
shows the levels of chemokine recovered from the BAL fluid before and 24 h after segmental allergen challenge as measured by ELISA. Each symbol
represents an individual subject (corresponding to those in Table I) with the black bar representing the mean.
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CHEMOKINE RECEPTORS ON HUMAN ASTHMATIC AIRWAY T CELLS
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FIGURE 7. CCR6 and CXCR3 ligands induce internalization of extracellular CCR6 or CXCR3 receptors but produce no change in total levels of
chemokine receptor. A, CD4⫹ BAL T cells were stained for either CCR6, CXCR3, or CCR4 (either as an extracellular receptor above or as total receptor
in permeabilized cells below) in the presence or absence of cognate ligands. Representative data is shown for one subject. B, Change in expression of CCR6,
CXCR3, or CCR4 is shown as the ratio of the geometric mean fluorescence intensity (gmfi): (gmfi of chemokine receptor ⫹ ligand)/(gmfi of chemokine
receptor without ligand added). Summary of chemokine receptor expression from extracellular staining is shown above and from total expression in
permeabilized cells is shown below. Bar graphs include data from three subjects ⫾ SEM.
addition of PMA and ionomycin altered this pattern of cytokine
production to a more Th1/Th1-type profile (Fig. 5C). With stimulation, the percentage of IFN-␥-producing PB and BAL T cells
was increased dramatically, whereas the percentage of IL-4-producing PB and BAL T cells increased modestly or was unchanged.
This suggests that a subset of BAL T cells may be activated to produce IL-4 or IFN-␥ at baseline and the total number of cytokine-
producing BAL T cells increase following challenge. With the addition of exogenous T cell stimulation, the BAL T cells display
increased skewing toward a Th1 profile, consistent with a higher percentage of T cells with IFN-␥-producing potential. The addition of
PMA and ionomycin induces signaling downstream of the TCR and
is likely to reveal T cell cytokine potential rather than actual cytokine
production following allergenic encounter. Because Th2 cytokines are
The Journal of Immunology
critical to the asthmatic response, IL-4 production observed in the
absence of exogenous stimulation may be associated with increased
baseline Th2 activity in asthmatics.
Memory markers on prechallenge PB and BAL and
postchallenge BAL
Chemokine expression in BAL is increased following segmental
allergen challenge
To understand which ligands might recruit CD4⫹ and CD8⫹ T
cells to the asthmatic lung, BAL fluid was examined before and
24 h following segmental allergen challenge for production of specific chemokine ligands (Fig. 6). It has been previously demonstrated that human BAL fluid is diluted ⬃100-fold during bronchoscopy, so we would predict that actual chemokine levels would
be ⬃100-fold higher in vivo than the values measured (20).
CCL20 (CCR6 ligand) and CXCL8 (CXCR1/2 ligand) were significantly increased following allergen challenge. In addition,
CXCL9, CXCL10, and CXCL11 (CXCR3 ligands); CCL17 and
CCL22 (CCR4 ligands); CCL2 (CCR2 ligand) were increased following segmental allergen challenge but did not reach statistical
significance. CCL11 and CCL26 (CCR3 ligands), CCL5 (CCR1,
3, 5 ligand), and CXCL16 (CXCR6 ligand) were relatively unchanged following allergen challenge. The increase in ligand production following segmental allergen challenge suggests that
CCR2, CCR4, CCR6, CXCR1/2, and CXCR3 may play important
roles in recruitment of cells to the asthmatic lung. In addition, the
decreased expression of CCR6 and CXCR3 on CD4⫹ and CD8⫹
BAL T cells following segmental allergen challenge may be due to
internalization of these receptors through engagement with cognate ligand (Fig. 6).
CCR6 and CXCR3 on CD4⫹ BAL T cells are internalized
following encounter with cognate ligand in vitro
To determine whether CCR6, CXCR3, and CCR4 ligands could
induce internalization and whether this affected CCR6, CXCR3,
and CCR4 surface levels, prechallenge CD4⫹ BAL T cells were
used in an in vitro internalization assay (Fig. 7). CD4⫹ BAL T
cells were incubated for 30 min with no ligand or cognate ligand
at various concentrations and stained for CCR6, CXCR3, or
CCR4, respectively. Extracellular CCR6 was down-regulated, but
total CCR6 levels stayed the same following incubation with increasing levels of its cognate ligand, CCL20. Similarly, extracellular CXCR3 was down-regulated when incubated with either
CXCL10 or CXCL11, but total CXCR3 was not altered following
incubation with ligand. CXCL11 was a more potent inducer of
CXCR3 internalization than CXCL10, similar to our previously
published data (21). For comparison, we examined extracellular
CCR4 internalization and found that CCL22 was dominant over
CCL17 in inducing internalization as previously shown (22) but
induced smaller levels of internalization with no significant
changes in total CCR4 levels. In addition, it is interesting to note
that CCR4 is found at similar surface and total levels, while surface and total CCR6 and CXCR3 are discordant, suggesting different mechanisms of surface receptor regulation in vivo. These
data argue that CCR6 and CXCR3 ligands in the BAL could induce internalization and be responsible for observed decreases in
BAL T cell CCR6 and CXCR3 expression following segmental
allergen challenge, while CCR4 ligands in the BAL induce more
subtle changes in BAL T cell CCR4 expression.
Discussion
In our study, we examined the phenotype and recruitment of human T cells to the allergic lung and revealed novel biology for
understanding the human asthmatic response. At baseline, we
found that specific chemokine receptors, including CCR1, CCR5,
CCR6, CCR9, CXCR1, CXCR2, CXCR3, CXCR4, CXCR6, and
BLT1 were significantly increased on CD4⫹ BAL T cells as compared with CD4⫹ PB T cells. CCR5, CCR6, and BLT1 were significantly increased on CD8⫹ BAL T cells as compared with
CD8⫹ PB T cells. In addition, we examined for the first time the
chemoattractant receptor profile on both CD4⫹ and CD8⫹ BAL T
cells before and 24 h following segmental allergen challenge. Although we predicted that we would observe an increase in IL-4producing T cells and Th2-associated chemoattractant receptors
(CCR3, CCR4, and CCR8) following airway challenge, we did not
observe a preferential enrichment of Th2 cells or Th2-associated
receptors. Surprisingly, we found that no receptors were significantly enriched but rather that CCR6 and CXCR3 were significantly decreased on both CD4⫹ and CD8⫹ BAL T cells
following challenge at 24 h. We did not rule out the significance
of other chemoattractant receptors in BAL T cell recruitment
but focused on understanding why CCR6 and CXCR3 were
down-regulated following challenge. Our data suggest that encounter with increased cognate ligand following challenge,
rather than alterations in Th1/Th2 cytokine balance or memory
phenotype, account for the decrease in CCR6 and CXCR3 on
BAL T cells and that CCR6 and CXCR3 play an important role
in propagating the human allergic asthmatic response.
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Although proliferation of pre-existing lymphocytes in the asthmatic lung may have occurred following segmental allergen challenge at 24 h, most of the lymphocytes would have to be recruited
from blood and other tissue sites to account for the ⬎15-fold average increase in lymphocytes, as demonstrated in murine studies
(16). To understand what combination of naive and memory T
cells were recruited, we phenotyped CD4⫹ and CD8⫹ PB and
BAL T cells pre- and postchallenge using the markers CD45RA
and CCR7 (Fig. 5, D–F). CD45RA was used to distinguish naive
vs memory T cells as studies have shown that loss of CD45RA
expression occurs as a T cell transitions from naive to memory
(17). In addition, we used CCR7 as a marker of lymph node homing potential as recent studies have shown that CCR7 defines T
cells with the capability of homing to lymph nodes from the tissue
via afferent lymphatics (18, 19). Thus, CD45RA and CCR7 provide important information about memory phenotype and lymph
node homing potential.
CD4⫹ T cells were divided into subsets: CD45RA⫹CCR7⫹ (naive), CD45RA⫺CCR7⫹ (CCR7⫹ memory), and CD45RA⫺CCR7⫺
(CCR7⫺ memory) (Fig. 5, D and F). Fewer naive and more CCR7⫺
memory CD4⫹ T cells were present in prechallenge BAL (as a percentage) as compared with either prechallenge PB or postchallenge
BAL, while the CCR7⫹ memory CD4⫹ T cell population was relatively unchanged between prechallenge PB and pre- and postchallenge BAL. CD8⫹ T cells were divided into similar subsets as
the CD4⫹ T cells: CD45RA⫹CCR7⫹ (naive), CD45RA⫺CCR7⫹
(CCR7⫹ memory), CD45RA⫺CCR7⫺ (CD45RA⫺CCR7⫺ memory), and CD45RA⫹CCR7⫺ (CD45RA re-expressing CCR7⫺ memory) (Fig. 5, E and G). Fewer naive, more CCR7⫹ memory, and
CD45RA⫺CCR7⫺ memory CD8⫹ T cells were present in prechallenge BAL as compared with prechallenge PB or postchallenge BAL,
while the CD45RA re-expressing CCR7⫺ memory CD8⫹ T cell population was relatively unchanged. Because the distribution of CD4⫹
and CD8⫹ memory T cell populations were most similar between the
prechallenge PB and postchallenge BAL samples, these data suggest
that T cells are recruited uniformly from PB regardless of memory
phenotype and that both naive and memory populations are recruited
to the asthmatic lung.
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CHEMOKINE RECEPTORS ON HUMAN ASTHMATIC AIRWAY T CELLS
gut-associated (CCR9) chemoattractant receptors, certain receptors
are enriched on tissue-localized T cells as compared with PB T
cells, including but not limited to CXCR3, CXCR6, CCR5, and
CCR6. For example, CXCR3, CXCR6, and CCR5 are highly enriched on liver T cells, whereas CCR6 and CXCR6, but not
CXCR3 or CCR5, are enriched on normal skin T cells (32, 33).
These receptors may play a role in homing to tissue sites or be
associated with memory T cells, which are enriched in the tissue.
Because healthy controls and asthmatic subjects express similar
chemoattractant receptors on BAL T cells before allergen challenge, we focused on differences in chemoattractant receptor expression on BAL T cells and chemokine production following segmental allergen challenge.
Another recent segmental allergen challenge study found that
CCR4 and CCR7 were increased and CXCR3 decreased as a percentage on bulk BAL T cells 42 h following allergen challenge but
only when selecting for the three subjects with highest eosinophilia
(28). The difficulty in comparing our study with this study (28) is
that specific chemokine receptors are expressed differentially on
CD4⫹ and CD8⫹ T cells, including but not limited to CXCR3,
CCR4, CCR5, CCR6, CXCR6, and CCR7. For instance, because
CCR4 is expressed almost exclusively on CD4⫹ T cells, increases
in the percentage of CCR4 on total BAL T cells may actually mark
an increase in CD4⫹ T cells as compared with CD8⫹ T cells. This
implies that grouping all CD3⫹ T cells together may mask (or
amplify) alterations in the chemokine receptor profile due to differences in the CD4-CD8 ratio in the BAL and PB.
Panina-Bordignon et al. (34) found a significant increase in the
total number of CCR4⫹ and CCR8⫹ T cells in bronchial biopsies
from allergen-challenged, as compared with sham-challenged,
asthmatics. We also found an increase in total CCR4⫹CD4⫹ T
cells (like most chemoattractant receptor positive CD4⫹ or CD8⫹
T cells) but noted that the percentage of CD4⫹ or CD8⫹ T cells of
expressing CCR4 was unchanged following challenge. Differences
between our findings and those of Panina-Bordignon et al. (34)
may result from differences in staining technique (immunohistochemistry vs flow cytometry) and cell isolation from different tissue compartments (BAL vs bronchial biopsy).
Although Th2 cytokines play a critical role in setting up the
asthmatic response, it has been shown that Th2 cells are not the
predominant T cell present in the asthmatic BAL through intracellular cytokine staining (29, 30, 35). In addition to determining
the percentage of Th2 cells present before and after segmental
allergen challenge, we determined the percentage of Th1 cells
present in the asthmatic airway because IFN-␥ may play an important role in either increasing or decreasing the severity of the
asthmatic response (5, 6). After stimulating cells with PMA and
ionomycin, we observed that the percentage of IL-4-producing
BAL T cells was similar before and after segmental allergen challenge, while the percentage of IFN-␥-producing BAL T cells was
somewhat decreased following segmental allergen challenge, similar to a previous study (29, 36). We also noted that in the absence
of exogenous stimulation with PMA and ionomycin that the percentage of IL-4-producing BAL T cells was unchanged, but that
the percentage of IFN-␥-producing cells was decreased significantly as compared with stimulated BAL T cells. Because the percentage of IL-4-producing BAL Th2 cells was unchanged following segmental allergen challenge, it was not surprising that the
percentage of Th2-associated receptors on BAL T cells was also
unchanged.
Increases in some or all BAL Th2 cytokines have been measured following segmental allergen challenge (23, 37– 40). Because IL-4, IL-5, and IL-13 can be produced by other leukocytes,
including eosinophils, basophils, and mast cells (41, 42), increases
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Segmental allergen challenge is useful because it allows direct
observation of the responses to allergen that occur in the human
airway. In our studies, allergen-induced airway narrowing was followed by significant increases in the recovery of both lymphocytes
and eosinophils, as is known to occur in the course of an asthma
exacerbation. Although neutrophils were recruited into the BAL of
some allergen challenged subjects, the increase varied widely from
subject to subject and did not reach statistical significance. Recent
studies examining the time course of leukocyte infiltration following segmental allergen challenge demonstrated that lymphocyte
and neutrophil recruitment peaked at 18 h postchallenge, whereas
eosinophil and alveolar macrophage recruitment peaked at 42 h
(23). This suggests that the recruitment of lymphocytes may have
reached its apex at 24 h postchallenge, while eosinophil numbers
are likely to accumulate beyond this time point.
A recent report has suggested that CD1d-restricted NKT cells
comprise the majority (⬎60%) of T cells in the asthmatic BAL as
compared with healthy controls or subjects with sarcoidosis (3).
We found that although CD1d-restricted NKT cells were significantly enriched in the BAL as compared with PB, they made up
only ⬍2.5% of the lymphocyte gate. Furthermore, we noted that
following segmental allergen challenge the percentage of BAL
CD1d-restricted NKT cells was unchanged from prechallenge levels. We believe that the discrepancy observed between our data
and the findings of Akbari et al. (3) is a result of nonspecific staining from alveolar macrophages in the BAL (14). Akbari et al. (3)
gated on CD3, which we believe led to nonspecific background
staining and artificially inflated numbers of BAL CD1d-restricted
NKT cells. This interpretation was supported by Vijayanand et al.
(24) who demonstrated that improper gating can lead to artificially
high numbers of CD1d-restricted NKT cells in the BAL. Our data
describing low numbers of BAL NKT cells was recently confirmed
by studies showing similar low numbers of BAL NKT cells in
persons with mild, moderate, and severe refractory asthma and in
healthy controls (24 –26). Further, Vijayanand et al. (24) found that
NKT cells were not preferentially enriched in the asthmatic airway
as they found the same low number of CD1d-restricted NKT cells
in airways of normal controls and subjects with chronic obstructive
pulmonary disease as they did in subjects with asthma (24). Thus,
while we found that CD1d-restricted NKT cells are enriched 10fold in the BAL as compared with PB, this appears not to be
specific to the asthmatic airway but more a reflection of a propensity for NKT cells to reside in the tissue. This is consistent with
what we found following Ag challenge, in which the percentage of
NKT cells in the lymphocyte gate was not increased. These data
also argue against preferential recruitment of CD1d-restricted
NKT cells into the asthmatic lung. We have previously demonstrated that CCR6 and CXCR3 are highly expressed on CD1drestricted NKT cells and could allow for recruitment into tissue
sites such as the lung, but these receptors would not be expected
to support the ⬎1000-fold enrichment in the BAL suggested by
Akbari et al. (3). Although CD1d-restricted NKT cells may contribute to the asthmatic response through secretion of Th2 cytokines, conventional T cells make up the predominant T cell
population in the asthmatic BAL and likely play the predominant role in promoting the asthmatic response.
It has been shown that similar chemokine receptor expression
profiles are found on BAL T cells from healthy controls and asthmatic subjects (27–31), so the increased expression of specific chemokine receptors on BAL T cells as compared with PB T cells is
likely to be related to both an increase in memory T cells in the
BAL as compared with PB and to the requirement for specific
chemoattractant receptors in trafficking to the BAL and other tissue
sites. In addition to the skin-associated (CCR4 and CCR10) and
The Journal of Immunology
seem to induce any alterations in CCR4 expression on CD4⫹ or
CD8⫹ BAL T cells. CCL22 has been shown to be a potent inducer
of CCR4 internalization as opposed to CCL17, so it is not clear
why CCR4 levels were not also down-regulated on CD4⫹ BAL T
cells following allergen challenge (22). This may be related to
lower concentrations of CCR4 ligands found in the BAL as compared with other chemoattractant levels or to rapid recycling of
CCR4 to the surface following internalization as opposed to CCR6
and CXCR3.
Our results, in conjunction with other published literature, suggest that recruitment of T cells following allergen encounter is
controlled sequentially by several distinct chemoattractant receptor-mediated pathways. During the earliest phase of allergen encounter, mast cells degranulate and release lipid and protein chemoattractants, such as BLT1 and CCR8 ligands, initiating
recruitment of Th2 cells along with other effector T cell populations (47, 48). Following this early phase, CCR4 ligands are produced following IL-4 and IL-13 induction of the STAT6 pathway
and lead to amplification of Th2 recruitment and the asthmatic
response (9).
In addition to these chemoattractant receptors, our data suggest
that CCR6 and CXCR3 play a critical role in propagating the asthmatic response. Data in mouse models of asthma suggest that increases in recruitment of CXCR3⫹ T cells may increase the severity of the asthmatic response (49) and that CCR6 is required for
the asthmatic response (50). Recently, Acosta-Rodriguez et al. (51)
identified CCR6 as a marker of Th17 cells. Although we did not
evaluate IL-17 our study, our finding that CCR6 is highly expressed on BAL T cells and down modulated after antigen challenge, suggests that Th17 cells may play a role in human asthma.
CCR6 and CXCR3 ligands are produced in response to direct TLR
and/or cytokine activation and induce recruitment of inflammatory
T cells that can amplify the asthmatic response (52, 53). TLR
stimulation during the asthmatic response can occur through TLR
agonists present in aeroallergens, such as in animal dander or dust
mites, or through TLR agonists present in respiratory viruses,
which are known to exacerbate asthma (54, 55). In conclusion, our
data provide support for additional chemoattractant targets in the
human asthmatic response and suggest that CCR6 and CXCR3
play an underappreciated role in T cell recruitment to the
asthmatic lung.
Acknowledgments
We thank Sandra Hong and Carol Leary for their technical assistance.
Disclosures
The authors have no financial conflict of interest.
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(45, 46). In terms of T cell chemoattractants, CCR4 ligands
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