A critical role for CCR2/MCP-1 interactions in the development of idiopathic pneumonia syndrome after allogeneic bone marrow transplantation

doi:10.1182/blood-2003-08-2708

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Blood, 15 March 2004, Vol. 103, No. 6, pp. 2417-2426.
Prepublished online as a Blood First Edition Paper on November 13, 2003; DOI 10.1182/blood-2003-08-2708.

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TRANSPLANTATION
A critical role for CCR2/MCP-1 interactions in the development of idiopathic pneumonia syndrome after allogeneic bone marrow transplantation
Gerhard C. Hildebrandt, Ulrich A. Duffner, Krystyna M. Olkiewicz, Leigh A. Corrion, Nicole E. Willmarth, Debra L. Williams, Shawn G. Clouthier, Cory M. Hogaboam, Pavan R. Reddy, Bethany B. Moore, William A. Kuziel, Chen Liu, Gregory Yanik, and Kenneth R. Cooke
From the Department of Internal Medicine and Pediatrics, Division of Hematology and Oncology, Blood and Marrow Transplantation Program, the Department of Internal Medicine, Division of Pulmonology and Critical Care, and the Department of Pathology, University of Michigan, Ann Arbor, MI; the Department of Pathology, University of Florida School of Medicine, Gainesville, FL; and Section of Molecular Genetics and Microbiology, The University of Texas, Austin.

   Abstract

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Idiopathic pneumonia syndrome (IPS) is a major complicationafter allogeneic bone marrow transplantation (allo-BMT) andinvolves the infiltration of donor leukocytes and the secretionof inflammatory cytokines. We hypothesized that leukocyte recruitmentduring IPS is dependent in part upon interactions between chemokinereceptor 2 (CCR2) and its primary ligand monocyte chemoattractantprotein–1 (MCP-1). To test this hypothesis, IPS was inducedin a lethally irradiated parent $->$ F₁ mouse BMT model. Comparedwith syngeneic controls, pulmonary expression of MCP-1 and CCR2mRNA was significantly increased after allo-BMT. Transplantationof CCR2-deficient (CCR2^-/-) donor cells resulted in a significantreduction in IPS severity compared with transplantation of wild-type(CCR2^+/+) cells and in reduced bronchoalveolar lavage (BAL)fluid cellularity and BAL fluid levels of tumor necrosis factor– ${alpha}$ (TNF- ${alpha}$ ) and soluble p55 TNF receptor (sTNFRI). In addition, neutralizationof MCP-1 resulted in significantly decreased lung injury comparedwith control-treated allogeneic recipients. Experimental datacorrelated with preliminary clinical findings; patients withIPS have elevated levels of MCP-1 in the BAL fluid at the timeof diagnosis. Collectively, these data demonstrate that CCR2/MCP-1interactions significantly contribute to the development ofexperimental IPS and suggest that interventions blocking thesereceptor-ligand interactions may represent novel strategiesto prevent or treat this lethal complication after allo-BMT.

   Introduction

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Allogeneic bone marrow transplantation (allo-BMT) has emergedas an important treatment for several malignant and nonmalignantdiseases. Unfortunately, the success of allo-BMT is limitedby serious complications. In particular, diffuse lung injuryoccurs in 25% to 55% of allo-BM transplant recipients and significantlycontributes to morbidity and mortality after BMT.^1-4 Historically,approximately 50% of all pneumonias seen after BMT have beensecondary to infection, but the judicious use of broad-spectrumantimicrobial prophylaxis in recent years has tipped the balanceof pulmonary complications from infectious to noninfectiouscauses.⁵ Noninfectious lung injury that occurs in the acutesetting has been defined as idiopathic pneumonia syndrome (IPS).⁴A retrospective study from Seattle showed a lower incidenceand earlier onset of IPS than previously reported, but the typicalclinical course involving the rapid onset of respiratory failureleading to death remained unchanged.⁶ A recent review from theUniversity of Michigan Medical Center demonstrated that thefrequency of IPS after allogeneic BMT ranged from 5% to 25%,depending upon donor source and the degree of antigenic mismatchbetween donor and recipient.⁷ Day-100 mortality was approximately80%, and the median time from the diagnosis of IPS to deathwas 13 days despite aggressive treatment with high-dose steroidsand broad-spectrum antimicrobial therapy.⁷
The pathophysiology of IPS is complex, and a significant bodyof clinical and experimental data has supported roles for bothallospecific donor T cells^8-10 and the production of inflammatorycytokines.^9,11-15 With respect to the latter, both hyporesponsivenessof donor cells to lipopolysaccharide (LPS) stimulation¹² andthe neutralization of tumor necrosis factor– ${alpha}$ (TNF- ${alpha}$ )¹¹result in decreased lung injury after BMT, underscoring theimportance of TNF- ${alpha}$ and donor monocytes and macrophages in thedevelopment of IPS.
Inflammatory chemokines are also produced in the lung duringmurine IPS.¹⁶ Interactions between chemokines and their receptorssignificantly contribute to leukocyte migration and leukocytefunction¹⁷ and are critical to both adaptive and innate immuneresponses. Chemokine receptor 2 (CCR2) is the receptor for monocytechemoattractant proteins (MCPs) 1 to 5 and is expressed on avariety of hematopoietic cells, including monocytes, macrophages,effector and memory T cells, B cells, natural killer (NK) cells,and immature dendritic cells.^18-22 MCP-1 (CC-chemokine ligand2 [CCL-2]; mouse JE) belongs to the CC-chemokine family, bindsspecifically to CCR2, and is important for monocyte, macrophage,and T-cell recruitment in several inflammatory models.^23-26MCP-1 is produced by hematopoietic, endothelial, epithelial,and smooth muscle cells in response to inflammatory stimulisuch as interleukin-1 ${beta}$ (IL-1 ${beta}$ ) and TNF- ${alpha}$ .^27-31 Abrogation of CCR2/MCP-1interactions, either by neutralization or deficiency of theligand or receptor, results in the impaired recruitment of monocytes,macrophages, and T cells in animal models of inflammatory andpulmonary diseases.^{23,24,26,32-37}
In light of the established role of donor accessory cells andlymphocytes in the development of IPS,^8-10,12 we examined thecontribution of CCR2/MCP-1 interactions to this process afterallo-BMT. We hypothesized that MCP-1 expression in the lungand CCR2 expression on donor leukocytes would have significantimpact on recruitment of monocytes, macrophages, and T cellsto the lung during IPS. Our results support this hypothesisand demonstrate that the expression of both MCP-1 and CCR2 issignificantly increased after allo-BMT. Furthermore, interruptionof CCR2/MCP-1 interactions after BMT, either by transplantationof CCR2^-/- donor cells or by neutralizing MCP-1, leads to significantreduction in lung injury, underscoring a critical role for thischemokine receptor/ligand pair in the development of IPS.

   Patients, materials, and methods

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Mice and bone marrow transplantation
Female B6D2F₁ (H-2^bxd), B6.C-H2 < bm1 > /ByJ (H-2^b), B6.C-H2< bm12 > KhEg (H-2^b), C57BL/6 (H-2^b), and B6-Ly5.2 (H-2^b)were purchased from Jackson Laboratory (Bar Harbor, ME) or fromthe Frederick Cancer Research and Development Center (NationalCancer Institute; Frederick, MD). CCR2^-/- mice³⁸ (B6129F2-Cmkbr2^tm1Kuz[H-2^b]) were bred at the University of Michigan (Ann Arbor,MI). In all analyses using CCR2^-/- mice, age-matched, CCR2^+/+B6.129PF2/J (H-2^b) (Jackson Laboratory) and C57BL/6 mice wereincluded as controls. Animals used for BMT and in vitro experimentswere at least 12 weeks old. All experiments were approved bythe University of Michigan Committee on the Use and Care ofAnimals.
Mice received BM transplants according to a previously describedprotocol.³⁹ When the haploidentical B6 $->$ B6D2F₁ system was used,cell mixtures of 5 x 10⁶ BM cells were supplemented with 2 x10⁶ splenic T cells from syngeneic (B6D2F₁) or allogeneic B6.129PF2/J,C57BL/6, B6-Ly5.2, or CCR2^-/- donors. T cell-purification wasperformed by either nylon wool nonadherence or CD4/CD8 magneticbead separation (autoMACS; Miltenyi Biotec, Bergisch Gladbach,Germany) according to the manufacturer's protocol. Approximately70% of cells obtained after nylon wool passage and more than85% of cells obtained by autoMACS were positive for CD4 or CD8(data not shown). Prior to transplantation, host mice received13 Gy total body irradiation (TBI) (¹³⁷Cs source) deliveredin 2 fractions separated by 3 hours. In the B6 $->$ bm1 BMT system,recipients received 11 Gy TBI, whereas in the B6 $->$ bm12 BMT system,recipients received 9 Gy TBI and 250 000 purified CD4⁺ T cells.Other transplantation parameters remained unchanged.
Bronchoalveolar lavage (BAL)
Mice were killed by exsanguination, and BAL was performed aspreviously described.⁴⁰ BAL fluid (BALF) supernatants were frozenfor subsequent analysis of cytokine and chemokine content, andcells were counted before being analyzed by flow cytometry orused for cytospin analysis.
Cytospin analysis
Aliquots of 50 000 cells were resuspended in 250 µL buffersolution, centrifuged at 162 g for 3 minutes onto Cytoslides(Thermo Shandon, Pittsburgh, PA), and stained by means of theDiff-Quik procedure (Dade Behring, Newark, DE) according themanufacturer's protocol. Cells were differentiated by morphologyinto lymphocytes, macrophages, monocytes, and neutrophils. Cellulardifferentials were determined for each sample by counting 300total cells and were performed in triplicate. Percentages foreach sample were then obtained by averaging the 3 results.
Cell surface phenotype analysis
Cells were stained with fluorescein isothiocyanate (FITC)–conjugatedmonoclonal antibodies (MoAbs) to CD45.1, CD45.2, and CD11b;phycoerythrin (PE)–conjugated CD4, CD8, and F4/80; orallophycocyanin (APC)–conjugated CD4 and CD8 as previouslydescribed.¹² All MoAbs were purchased from BD Pharmingen (SanDiego, CA). CCR2 staining was performed with goat antimouseCCR2 (Santa Cruz Biotechnology, Santa Cruz, CA) and FITC rabbitantigoat antibodies (Zymed, San Francisco, CA). Three-colorflow cytometric analysis was performed by means of a FACSCalibur(BD Biosciences, San Jose, CA). The FACScan was calibrated withthe use of FITC-, PE-, and APC-conjugated, nonspecific immunoglobulinG (IgG) antibodies.
Histopathology and immunohistochemistry
Lung histopathology was determined in BM transplant–recipientanimals at 1, 2, 3, 4, or 6 weeks after BMT as previously described.⁴⁰Immunohistochemical staining was performed with antimouse MCP-1/JEantibody (R&D Systems, Minneapolis, MN) or goat IgG isotypecontrol (Sigma-Aldrich, St Louis, MO) (both 1:200 dilution)and the Vectastain ABC-AP Kit (Vector Laboratories, Burlingame,CA) plus Fast Red Tablets (Bio-Genex, San Ramon, CA) accordingto the manufacturer's protocol.
Cell function assays
To assess alveolar macrophage TNF- ${alpha}$ production in vitro, BALFcells from naive CCR2^+/+ and CCR2^-/- animals were normalizedfor alveolar macrophages by cytospin analysis. First, 5 x 10⁴macrophages were plated per well in 96-well plates (Falcon,BD Labware, Lincoln Park, NJ) with or without stimulation withLPS (5 to 100 ng/mL). After 4 hours, supernatants were analyzedfor TNF- ${alpha}$ by enzyme-linked immunosorbent assay (ELISA). To determineTNF- ${alpha}$ production of pulmonary macrophages after BMT, lung cellswere harvested from mice at week 6 as previously described,¹²normalized for monocytes/macrophages by cytospin analysis, platedat 5 x 10⁴ monocytes/macrophages per well, and finally stimulatedand assessed for TNF- ${alpha}$ secretion by ELISA. To measure T-cellproliferation in response to alloantigen, 2 x 10⁵ B6 CCR2^+/+or CCR2^-/- splenic T cells were cultured for 120 hours in thepresence of 1 x 10⁵ irradiated (20 Gy) naive allogeneic (B6D2F₁)or syngeneic (B6) peritoneal cells. After 96 hours, supernatantwas analyzed for interferon- ${gamma}$ (IFN- ${gamma}$ ) and TNF- ${alpha}$ . Determinationof T-cell proliferation and cytolytic function were completedas previously described.⁴¹ For in vivo cytokine production,serum was collected 5 and 21 days after BMT and analyzed forTNF- ${alpha}$ and IFN- ${gamma}$ . Donor T-cell expansion was assessed 5 days afterBMT. Single-cell splenocyte suspensions were obtained from individualanimals, counted, and stained for CD4 and CD8.
RNase protection assay (RPA)
After perfusion of the pulmonary vascular system with ice-coldphospate-buffered saline (PBS), whole-lung tissue was retrievedat various time points after BMT and stored at -80°C. ThemRNA was extracted from whole lungs by means of TRIzol followingthe manufacturer's protocol (GibcoBRL, Grand Island, NY) andquantitated by spectrophotometry. The multiprobe template setsmCK-5b and mCR-5 were purchased from BD Pharmingen. [³²P]uridine(5')-triphosphate (UTP)–radiolabeled antisense riboprobeswere synthesized according to the manufacturer's protocol andpurified by means of G-25 Sephadex Quick Spin Columns (Roche,Indianapolis, IN). Expression of chemokine genes was quantifiedby RPA with the use of RiboQuant RPA kits (BD Pharmingen) accordingto the manufacturer's protocol. Protected RNA products wereseparated on a 5% polyacrylamide gel; the gel was exposed toa storage phosphor screen (Molecular Dynamics, Sunnyvale, CA)for quantification. Signal intensity was measured with ImageQuant(MolecularDynamics) and standardized to the intensity of the L32 signalfor each sample.
Cytokine ELISA
ELISA kits for MCP-1 (BioSource, Camarillo, CA), IFN- ${gamma}$ (BD Pharmingen),TNF- ${alpha}$ (R&D Systems for cell culture supernatants; BioSourcefor BALF), and soluble p55 TNF receptor (sTNFRI) (R&D Systems)were used to measure concentrations of the proteins. Assayswere performed according to the manufacturer's protocol.
Anti–MCP-1 treatment
In some experiments, BM transplant recipients were treated withpolyclonal antibodies against MCP-1 or with preimmune serum.⁴²The antiserum containing polyclonal Abs directed against mouseMCP-1/CCL2 was generated in New Zealand White rabbits by meansof a well-established protocol.⁴³ The specificity of the anti–MCP-1/CCL2antiserum was rigorously screened before its use in an experiment,and it lacked cross-reactivity with other chemokines and cytokines.⁴²Allo-BM transplant recipients were injected intraperitoneallywith 250 µL either anti–MCP-1 antibodies (titersof 10⁷/mL) or preimmune serum on days 10, 12, 16, 20, 24, and28 after transplant. Syngeneic BM transplant recipients receivedonly preimmune serum or were left untreated.
BALF MCP-1 levels in BM transplant recipients and healthy volunteers
BALF samples analyzed for MCP-1 levels were obtained from BMtransplant recipients with either acute (IPS) or chronic noninfectiouspulmonary dysfunction and from healthy volunteers. BALF wascollected in a systematic manner in all BM transplant recipients.A total volume of 2 mL/kg sterile saline (maximum volume, 180mL) was instilled into the patient's lungs. Collected BALF waspooled, divided into aliquots, and frozen for subsequent analysis.BALF MCP-1 protein levels were measured by means of a humanMCP-1 ELISA kit (BD Pharmingen) according to the manufacturer'sprotocol. All samples were run in duplicate, and the sensitivityof the assay was 15 pg/mL.
Statistical considerations
All values are expressed as the mean ± standard errorof the mean (SEM). The parametric independent sample t testwas used for statistical comparisons between groups unless thenumber of samples was lower than 5, in which case the nonparametricMann-Whitney test was used. The Wilcoxon rank test was usedfor analyzing survival data.

   Results

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Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

Donor monocytes/macrophages and T cells migrate into the lung and cause lung injury after allogeneic BMT
Lethally irradiated B6D2F₁ mice received BM transplants withsyngeneic (B6D2F₁) or allogeneic (B6 Ly5.2) bone marrow and2 x 10⁶ donor T cells. Animals were analyzed for lung histopathologyand BALF cellularity at 1, 2, 4, and 6 weeks after transplantation.Consistent with previous work using other strain combinations,^12,40mice receiving syngeneic BM transplants maintained normal histologyat each time point (Figure 1A), whereas recipients of allo-BMtransplants developed significant lung injury (Figure 1B). Semiquantitativeevaluation of lung sections demonstrated that significant pulmonarydamage was first detected 2 weeks after allo-BMT and progressedover time (Figure 1C). Analysis of BALF cellularity demonstratedthat the severity of lung histopathology correlated with increasingnumbers of inflammatory cells in the bronchoalveolar space (Figure 1D-E).

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Figure 1.. Recruitment of donor effector cells to the lungs after BMT. Donor T cells and monocytes/macrophages are recruited to the lung and cause lung injury after allogeneic BMT. B6D2F₁ mice received allogeneic ( ${blacksquare}$ ) or syngeneic ( ${square}$ ) BM transplants, and lungs were examined at weeks 1, 2, 4, and 6 as described in "Patients, materials, and methods." Photomicrographs (original magnification, x 200) from hematoxylin-eosin–stained sections obtained 6 weeks after syngeneic (panel A) or allogeneic (panel B) BMT. Recipients of allogeneic BM transplants develop significant lung pathology compared with syngeneic controls as determined with a semiquantitative scoring system (panel C). Total BAL fluid cellularity (panel D) and T-cell counts (panel E) correlate with histologic changes. Data are from 2 experiments representative of 3 and are presented as mean ± SEM; n = 8 to 10 per group per time point; ^*P < .01.

We next investigated the kinetics of donor leukocyte chimerismin the lung by using congenic B6 donors that express the CD45.1allele for the polymorphic region of the common leukocyte antigen(CD45). B6D2F₁ recipients express the CD45.2 allele. BALF cellswere collected at 1, 2, and 4 weeks after BMT and analyzed byflow cytometry after staining with CD45.1, CD45.2, and eitherF4/80 (macrophages) or CD4 and CD8 (T cells). When donor T-cellrecruitment to the lung was evaluated, we found that the majorityof CD4⁺ and CD8⁺ T cells in the BALF were of donor origin asearly as day 7, and that turnover was complete by day 14. Bycontrast, donor macrophage recruitment occurred more slowly;only 10% of macrophages were of donor origin on day 7, and turnoverwas not complete until 4 weeks after BMT (data not shown).
MCP-1 levels in the lung are increased after allo-BMT
MCP-1 as well as other inflammatory chemokines, like regulatedon activation, normal T cell expressed and secreted (RANTES)and macrophage inflammatory protein 1 ${alpha}$ (MIP-1 ${alpha}$ ), can be inducedby inflammatory mediators like TNF- ${alpha}$ and LPS,²⁷ both of whichcontribute to the development of IPS.^11,12,40 We therefore hypothesizedthat pulmonary expression of inflammatory chemokines, includingMCP-1, would be increased after allo-BMT. RNA was isolated fromlungs at weeks 1, 2, 4, and 6 after BMT. Using RPA, we foundthat mRNA expression of RANTES, MIP-1 ${alpha}$ , MIP-1 ${beta}$ , and MCP-1 wasincreased in the lungs of allogeneic recipients (Figure 2A).MCP-1 mRNA was increased as early as week 1 (12.7-fold comparedwith naive), reached its maximal expression by week 2 (21.3-fold),and then declined over time until week 6 after transplantation.At all time points, MCP-1 mRNA expression was higher in allogeneicanimals than in syngeneic controls (Figure 2A-B). PulmonarymRNA expression of MCP-1 after allo-BMT correlated with increasesin BALF MCP-1 protein levels at weeks 2 and 6 after BMT andwith enhanced MCP-1 expression in the lung tissue as determinedby immunohistochemistry (Figure 2C-E).

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Figure 2.. Increase in MCP-1 levels in the lung after allogeneic BMT. Animals received allogeneic ( ${blacksquare}$ ) or syngeneic ( ${square}$ ) BM transplants as in Figure 1. (A) MCP-1 mRNA expression was determined after BMT by RNAase protection assay. (B) MCP-1 expression is increased after allogeneic BMT compared with syngeneic controls at all time points. (C) BALF protein levels of MCP-1 (ELISA) are increased at week 2 and week 6 after allogeneic BMT. Data are presented as mean ± SEM; n = 3 to 10 animals per group; ^*P < .01. (D-E) Immunohistochemical alkaline phosphatase staining for MCP-1 in lungs from syngeneic (left) and allogeneic (right) BM transplant recipients 14 days after transplantation. Original magnifications: x 200 (D); x 400 (E).

Pulmonary CCR2 mRNA expression is increased after allo-BMT and correlates with lung pathology
CCR2 is expressed on monocytes, macrophages, and T cells²¹ andcontributes to the recruitment of these cells in various modelsof disease.^23,24,26,32 The expression of CCR2 mRNA was measuredat weeks 1, 2, 4, and 6 after BMT. Pulmonary CCR2 mRNA expressionwas elevated in allogeneic animals compared with syngeneic controlsby week 2, continued to rise over time (Figure 3A), and correlatedwith increasing lung histopathology and BALF cellularity (compareFigure 1). By gating on monocytes/macrophages or costainingwith F4/80, fluorescence-activated cell sorter (FACS) analysisof BALF cells demonstrated increases in protein expression ofCCR2 and in the percentage of CCR2⁺ cells after allo-BMT (Figure 3B).In addition, a higher percentage of F4/80⁺ macrophagesalso coexpressed CD11b (Figure 3C), consistent with a previouslydescribed phenotype of newly recruited alveolar macrophages.^44,45

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Figure 3.. Recruitment of CCR2⁺ cells to the lung after allogeneic BMT. Animals received BM transplants as in Figure 1. CCR2 mRNA was determined after BMT by RNase protection assay. (A) CCR2 mRNA expression in the lungs of allogeneic recipients ( ${blacksquare}$ ) was elevated by week 2 and continued to rise over time through week 6 compared with syngeneic controls ( ${square}$ ). Data are presented as mean ± SEM and are from 3 to 6 animals per group. (B) CCR2 protein expression is increased on monocytes and macrophages recruited to the alveolar space after allogeneic BMT. (C) F4/80⁺ macrophages in the BALF show a phenotype previously described for newly recruited monocytes to the alveolar space (F4/80⁺/CD11b⁺).^44,45 Thin line indicates isotype control; open histogram, syngeneic; and shaded histogram, allogeneic.

Lung injury is decreased in recipients of allogeneic CCR2^-/- donor cells
To determine the role of CCR2 expression in the developmentof IPS, B6D2F₁ mice received allo-BM transplants from eitherCCR2^+/+ or CCR2^-/- donors. BMT parameters otherwise remainedunchanged, and syngeneic controls were again included. Allo-BMTwith CCR2^-/- donor cells resulted in a significant reductionin lung pathology by week 6 compared with allogeneic CCR2^+/+controls (Figure 4A-B), whereas graft-versus-host disease (GVHD)–associatedtarget organ injury to liver or gastrointestinal tract and survivalwere comparable in the 2 groups (Figure 4C; Table 1). Reducedlung injury was associated with decreases in total BALF cellularity(Figure 4D) and in the absolute numbers of BALF monocytes andmacrophages as determined by visual differential (Figure 4E)and by flow cytometric analysis for F4/80 and CD11b (data notshown). In addition, the percentage of F4/80⁺ cells coexpressingCD11b was significantly lower in recipients of CCR2^-/- BM transplantscompared with CCR2^+/+ controls, confirming a reduction in newlyrecruited macrophages to the alveolar space^44,45 (Figure 4F).BALF CD8⁺ and CD4⁺ T cells were also decreased after CCR2^-/-BMT although the decrease in CD4⁺ cells did not reach statisticalsignificance (Figure 4E). The reduction of cells recruited tothe lung after CCR2^-/- BMT was associated with a significantdecrease in pulmonary CCR2 mRNA expression (Figure 4G), supportingthe hypothesis that increases in CCR2 mRNA levels after allo-BMTreflect the infiltration of CCR2-expressing donor leukocytes.Residual CCR2 mRNA levels observed after CCR2^-/- BMT can beexplained by the ability of nonhematopoietic cells in the lungto express this receptor.^46-48

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Figure 4.. Development of less severe lung injury in recipients of CCR2-deficient donor cells after allogeneic BMT. Lethally irradiated B6D2F₁ mice received BM transplants from either allogeneic CCR2^+/+ ( ${blacksquare}$ ) or CCR2^-/- () or syngeneic ( ${square}$ ) donors as described in "Patients, materials, and methods," and animals were analyzed 6 weeks after BMT. (A) Photomicrographs of lung tissue 6 weeks after BMT (hematoxylineosin [HE]; original magnification, x 200). (B) (C) Lung injury was significantly reduced after allogeneic CCR2^-/- BMT compared with allogeneic CCR2^+/+ controls, whereas target organ injury to liver and gastrointestinal tract (SB = small bowel, LB = large bowel) and survival until time of analysis did not differ. Pathology data are presented from 1 experiment representative of 2; n = 5 to 7 per group; ^**P < .01. (D) (E) BALF cellularity (panel D) and absolute numbers of monocytes/macrophages and CD8⁺ T cells (panel E) were significantly decreased after CCR2^-/- BMT compared with allogeneic CCR2^+/+ BMT controls. Data presented are from 2 experiments representative of 4; n = 6 to 11 per group; ^*P < .05. (F) In addition to the total number of F4/80⁺ cells in the BALF, the percentage of F4/80⁺/CD11b⁺ cells was reduced in recipients of CCR2^-/- BM transplants. (G) CCR2 mRNA in the lungs was decreased 6 weeks after allogeneic CCR2^-/- BMT. (H) Reduced lung pathology and BALF cellularity correlated with significantly decreased levels of TNF- ${alpha}$ and sTNFRI in the BAL fluid. Data are pooled from 3 experiments; data are presented as mean ± SEM; n = 10 to 17 per group; ^*P < .05. (I) Lung pathology and BALF cellularity are reduced following allogeneic BMT with CCR2^-/- cells compared with allogeneic controls in isolated major histocompatibility complex (MHC) class I and class II disparate BMT systems. Data are presented as mean ± SEM and are from 1 of 2 comparable experiments; n = 3 to 5 per group;^*P < .05.

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Table 1.. Combined survival data from 6 transplant experiments

Monocytes, macrophages, and T cells are significant sourcesof TNF- ${alpha}$ after allo-BMT,^12,49,50 and TNF- ${alpha}$ is important in thedevelopment of IPS.^11,13,51,52 Furthermore, sTNFRI has beenshown to correlate with GVHD and other transplantation-relatedcomplications in humans.⁵³ We therefore measured BALF levelsof TNF and sTNFRI and found that both were decreased in recipientsof CCR2^-/- BM transplants compared with CCR2^+/+ controls (Figure 4H).Finally, similar reductions in IPS severity were seen withthe use of CCR2^-/- donors in the context of a single MHC classI (B6 $->$ bm1) or class II (B6 $->$ bm12) mismatch between donor andhost, demonstrating that the reduction in lung injury was nota strain-specific phenomenon (Figure 4I).
CCR2 deficiency of T cells and macrophages does not alter alloreactivity to host antigens or cytokine production
We hypothesized that the reduction in IPS severity after CCR2^-/-BMT was secondary to a defect in the recruitment of CCR2^-/-donor cells to the lung rather than from intrinsic defects incytokine production and alloreactivity of CCR2-deficient monocytes/macrophagesand T cells, respectively. To examine this possibility, we stimulatedalveolar macrophages from naive CCR2^-/- and CCR2^+/+ animalswith LPS in vitro as described in "Patients, materials, andmethods," and found no differences in TNF- ${alpha}$ production in the2 groups (Figure 5A). Similar findings were noted ex vivo; pulmonarymonocytes and macrophages isolated from recipients of eitherCCR2^-/- or CCR2^+/+ allo-BM transplants produced comparable amountsof TNF- ${alpha}$ when stimulated with LPS (Figure 5B). Furthermore, whencompared with CCR2^+/+ cells, naive CCR2^-/- T cells showed nodifferences in proliferation or in IFN- ${gamma}$ and TNF- ${alpha}$ secretion (whenstimulated in a mixed lymphocyte reaction) or in cytolytic function(Figure 5C-F). Finally, no differences were observed betweenallogeneic groups when T-cell expansion and systemic IFN- ${gamma}$ andTNF- ${alpha}$ levels were measured after BMT (Figure 5G-I).

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Figure 5.. Effect of CCR2 deficiency in macrophages and T cells on cytokine production or alloreactivity to host antigens. CCR2 deficiency of macrophages and T cells does not impair cytokine production or alloreactivity to host antigens in vitro and in vivo. (A) Naive alveolar macrophages of CCR2^+/+ ( ${blacksquare}$ ) or CCR2^-/- () mice were stimulated in vitro for 4 hours with different concentrations of LPS, and TNF- ${alpha}$ levels in the supernatant were determined by ELISA. (B) Pulmonary macrophages were harvested 6 weeks after CCR2^+/+ ( ${blacksquare}$ ), CCR2^-/- (), or syngeneic ( ${square}$ ) BMT and stimulated with LPS in vitro; ^*P < .01. (C) (D) (E) Allo-specific proliferation (panel C) and in vitro IFN- ${gamma}$ (panel D) and TNF- ${alpha}$ (panel E) production were assessed in a mixed lymphocyte reaction with CCR2^+/+ ( ${blacksquare}$ ) or CCR2^-/- () T cells and allogeneic B6D2F₁ stimulators or with CCR2^+/+ ( ${square}$ ) T cells and syngeneic B6 stimulators. (F) Cytotoxic function of T cells was determined by an alloantigen-specific cytotoxic T lymphocyte (CTL) assay using P-815 (H2^d) and EL-4 (H2^b) target cells as described ( ${blacksquare}$ , CCR2^+/+ $->$ P-815; ${bullet}$ , CCR2^-/- $->$ P-815; ${blacktriangleup}$ , CCR2^+/+ $->$ EL-4; ${diamondsuit}$ , CCR2^-/- $->$ EL-4). All data presented are from 1 experiment representative of 3. (G) (H) (I) No differences in splenic T-cell expansion, serum IFN- ${gamma}$ , or serum TNF- ${alpha}$ levels were observed after allogeneic CCR2^+/+ ( ${blacksquare}$ ) or CCR2^-/- () BMT, and measurements in both allogeneic groups were greater than in syngeneic controls ( ${square}$ ). Data are presented as mean ± SEM from 1 of 2 comparable experiments; n = 4 to 5 per group; ^*P < .01.

In vivo neutralization of MCP-1 after allo-BMT reduces the severity of IPS
We next determined the effects of in vivo neutralization ofMCP-1 on the development of IPS. B6D2F₁ recipient mice receivedeither syngeneic or allogeneic BM transplant as described inFigure 1. Allo-BM transplant recipients were injected intraperitoneallywith 250 µL of either polyclonal anti–MCP-1 antibodiesor control serum starting on day 10 after transplantation asdescribed in "Patients, materials, and methods." We chose thisschedule in order to block MCP-1 prior to peak expression ofpulmonary mRNA levels and the influx of donor mononuclear cellsto the lung. We also opted to avoid neutralizing MCP-1 in thesetting of severe systemic inflammation that is seen duringthe first week after allo-BMT, since a similar strategy provedto be deleterious in an animal model of sepsis.⁵⁴ Syngeneiccontrols received preimmune serum at the same volume and schedule.To exclude a potential nonspecific effect of rabbit serum, somesyngeneic controls received no treatment. All groups were analyzedby day 30 for lung histopathology and BAL fluid cellularity.MCP-1 neutralization had no effect on mortality (data not shown).Consistent with previous experiments in this system, allo-BMtransplant recipients receiving control serum developed significantlung injury, whereas immunoneutralization of MCP-1 resultedin significantly reduced IPS severity and BALF cellularity (Figure 6A-B).Administration of rabbit serum had no effect on lunghistopathology in syngeneic controls, nor were symptoms of serumsickness observed (data not shown).

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Figure 6.. Reduction in the severity of IPS by in vivo neutralization of MCP-1 after allogeneic BMT. Lethally irradiated B6D2F₁ mice received allogeneic CCR2^+/+ BM transplants and either control serum ( ${blacksquare}$ ) or anti–MCP-1 () as described in "Patients, materials, and methods." Syngeneic animals received control serum ( ${square}$ )or no treatment (data not shown). Neutralization of MCP-1 resulted in significant reductions in both lung injury (panel A) and BALF (panel B) cellularity compared with allogeneic animals treated with control serum. Data are presented as mean ± SEM and are pooled from 2 similar experiments; n = 8 to 13 per group; ^*P < .05.

MCP-1 levels are increased in the BAL fluid of patients with IPS after allogeneic BMT
In a final set of experiments, we measured MCP-1 levels in BALfluid obtained from BM transplant recipients who had eitheracute (IPS) or chronic noninfectious pulmonary dysfunction andwere enrolled on clinical protocols approved by the Universityof Michigan's Institutional Review Board (IRB) and from healthyvolunteers. IPS was diagnosed in adult and pediatric BM transplantrecipients (median age, 20 years; range, 1-43 years) if theyfulfilled criteria defined by Clark et al.⁴ IPS was diagnosedwithin 100 days (median, 12 days; range, 9-56 days) after receiptof full-intensity 5/6 (n = 1) or 6/6 (n = 10) human leukocyteantigen (HLA)–matched allogeneic BM transplants from eithera related (n = 2) or unrelated (n = 9) donor. All patients hadclinical and radiographic evidence of diffuse lung injury andno evidence of an active systemic (blood/urine) or lower respiratorytract infection as assessed by BAL at time of study entry. Patientswho required inotropic blood pressure support or in whom pulmonarydysfunction was believed to be secondary to heart failure orfluid overload were not included. Chronic pulmonary dysfunctionwas defined as obstructive lung disease (OLD) or restrictivelung disease (RLD) using the following parameters obtained fromat least 2 consecutive pulmonary function tests. OLD: forcedexpiratory volume in one second (FEV_1.0)/functional vital capacity(FVC) $<=$ 80% or FEV_1.0/FVC $>=$ 15% lower than valuesmeasured before BMT, RLD: FVC or total lung capacity (TLC) $<=$ 80% or $>=$ 15% lower than values measured beforeBMT. Patients whose baseline (pre-BMT) measurements for FEV_1.0/FVC,FVC or TLC were $<=$ 80% must have had a $>=$ 15% declinein values. Eligible patients were greater than 100 days afterBMT and had no evidence for active systemic or lower respiratorytract infection. BALF samples were collected at study entry,processed and assayed for MCP-1 as described in "Patients, materials,and methods." As shown in Figure 7, BALF MCP-1 levels were markedlyelevated in patients with IPS compared with patients with chronicpulmonary dysfunction and healthy controls.

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Figure 7.. Significant increase in BAL fluid levels of MCP-1 in patients with IPS after allogeneic BMT. BAL fluid was obtained from healthy volunteers (n = 5) and from allogeneic BM transplant recipients with IPS (n = 11) or chronic noninfectious lung injury (n = 14) after allogeneic BMT as described in "Patients, materials, and methods." Individual data points are expressed. Horizontal bars indicate the average value in each group. ^*P < .05, IPS and chronic versus healthy controls; ⁺P < .05, IPS versus chronic.

   Discussion

Top
Abstract
Introduction
Patients, materials, and methods
Results
Discussion
References

IPS remains a frequently fatal complication after allo-BMT.Risk factors for IPS have included conditioning with TBI, acuteGVHD, older recipient age, initial diagnosis of malignancy otherthan leukemia, and the use of methotrexate (MTX) for GVHD prophylaxis.^3,6,55-58The likelihood of developing IPS increases with the number ofidentified risk factors.² A recent report from Seattle, WA,found that despite greater patient age and a similar incidenceof acute GVHD, recipients of allogeneic BMT using nonmyeloablativeconditioning have a reduced risk of IPS compared with patientsreceiving myeloablative conditioning.⁵⁹ Once established, pulmonarytoxicity was severe in each group and resulted in respiratoryfailure in the majority of patients. These findings suggestthat the intensity of BMT conditioning plays an important rolein the development of IPS, and they are consistent with datagenerated from two mouse BMT models showing that the lung issensitive to the combined effects of radiation and alloreactiveT cells.^60,61
Potential etiologies for IPS include direct toxic effects ofBMT conditioning regimens, occult pulmonary infections, andthe release of inflammatory cytokines that have been implicatedin other forms of pulmonary injury.^62-64 Immunologic factorsmay also be important, as suggested by the association of IPSand allogeneic (versus autologous or syngeneic) BMT and severeGVHD (versus mild or no GVHD).^2,5,6,55,65 Acute GVHD often precedesIPS, suggesting a possible causal relationship between the twodisorders.^3,55,66,67 Although the consistent association betweenlung injury and GVHD after experimental BMT also supports suchan etiology,^8,9,13,40,52 the role of GVHD and, specifically,alloreactive donor T lymphocytes in the pathogenesis of IPSremains a topic of considerable debate. Epithelial apoptosisafter BMT is usually attributed to T-cell–mediated injuryand is considered pathognomonic for acute GVHD. While observedin the lungs of some patients with IPS,⁶⁸ epithelial apoptosishas not been consistently identified in allogeneic BM transplantrecipients with pulmonary dysfunction.^67,69,70 The heterogeneityof pulmonary histopathology after allogeneic BMT is furthercomplicated by the nonspecific changes that occur after mechanicalventilation and by the limited quality and quantity of lungbiopsy tissue.
Despite the lack of classic acute GVHD histopathology, severallines of evidence suggest that the lung is susceptible to a2-pronged immunologic attack involving both inflammatory cytokinesand cellular effector pathways. However, the mechanisms by whichactivated leukocytes traffic to the lung and cause inflammationafter allogeneic BMT remain unresolved. Leukocyte traffickingto sites of inflammation involves interactions with endothelialcells that are facilitated by adhesion molecules and by chemokinesand their receptors.⁷¹ Previous studies have demonstrated thatincreases in the expression of a variety of inflammatory chemokineligands and receptors are associated with the development ofIPS.^16,72 For example, the transfer of alloreactive T-helper1 (Th1) cells into nonirradiated recipient mice to induce pulmonaryinflammation was associated with increased expression of RANTES,MIP-1 ${alpha}$ , MIP-1 ${beta}$ , IP-10, and monocyte IFN- ${gamma}$ –inducible protein(Mig).⁷² In addition, analysis of chemokine expression in thelung of lethally irradiated recipients of fully mismatched BMtransplants revealed that protein and mRNA expression of MCP-1,MIP-1 ${alpha}$ , RANTES, C10, and IP-10 were elevated in the lung 7 daysafter transplantation.¹⁶ Despite these findings, a mechanisticrelationship between chemokines and recruitment of cells tothe lung during IPS has not been fully elucidated. Althougha role for MIP-1 ${alpha}$ in the recruitment of leukocytes to the lungafter BMT was noted in one report,⁷³ subsequent work by thesame group suggested that the use of MIP-1^-/- mice as allo-BMtransplant donors exacerbated rather than reduced early lunginjury.⁷⁴
We demonstrate that both donor T cells and accessory cells infiltratethe lung as histopathology progresses after allo-BMT; turnoverof donor T lymphocytes and macrophages in the bronchoalveolarspace is complete by weeks 2 and 4, respectively. We hypothesizedthat the chemokine receptor CCR2 and its principal ligand MCP-1are critical to the recruitment of these donor cells to thelung after allo-BMT. Our data support this hypothesis and demonstratethat pulmonary MCP-1 mRNA and protein levels are increased earlyafter transplantation and are followed by enhanced CCR2 expressionthat directly correlates with progressive cellular infiltrationinto the lung. Furthermore, transplantation of CCR2^-/- donorcells reduced the severity of IPS in several strain combinations.Neutralization of MCP-1 after BMT resulted in a significantdecrease in lung injury as well, and clinical studies demonstratethat this chemokine is significantly elevated in patients withIPS. Despite the protective effect in the lung, abrogation ofCCR2/MCP-1 interactions by either method did not significantlyreduce mortality or hepatic and intestinal inflammation afterallogeneic BMT. These findings are consistent with data fromothers showing that successful inhibition of mechanisms responsiblefor leukocyte trafficking can reduce lung injury without significantlyaltering other GVHD target organs or survival after allo-BMT.^72,75,76Previously, we showed that the severity of intestinal GVHD withinthe first week after BMT directly correlates with overall survival⁷⁷;it remains to be determined whether MCP-1 expression is increasedin the gastrointestinal tract early after transplantation. Moreover,recent work from our laboratory has shown that CXCR3 expressionis critical to T-cell recruitment to the gastrointestinal tract,⁷⁸suggesting that the contribution of chemokine receptor-ligandinteractions to GVHD induction may be target-organ dependent.
The decrease in lung injury seen after CCR2^-/- BMT was associatedwith significant reductions in BALF levels of TNF- ${alpha}$ and sTNFRI.TNF- ${alpha}$ has been shown to be a critical effector molecule in thepathogenesis of IPS; neutralization of TNF- ${alpha}$ reduces the progressionof lung injury after allo-BMT,^9,11 and the capacity of donoreffector cells to secrete TNF- ${alpha}$ in response to LPS stimulationpredicts the severity of IPS.¹² The p55 TNFR is constitutivelyexpressed on a variety of cell types, and its soluble form isderived via proteolytic cleavage of the membrane-bound proteinin response to a variety of inflammatory mediators, includingLPS and TNF- ${alpha}$ .^79,80 The sTNFRI levels are elevated in the BALfluid of patients with IPS,¹⁵ and enhanced serum levels correlatewith the development of GVHD and other complications after BMT.⁵³
The reduction in BAL fluid TNF- ${alpha}$ levels could have been secondaryeither to decreased recruitment of TNF- ${alpha}$ –producing cellsor to an intrinsic defect in cytokine secretion in CCR2-deficientleukocytes. We favor the former for the following reasons: (1)Using fluorescent antibody staining for cell surface antigensand intracytoplasmic TNF- ${alpha}$ , we have found that lymphocytes andmacrophages are the primary producers of TNF- ${alpha}$ in the lung afterBMT (data not shown). (2) Allo-BMT with CCR2^-/- cells resultedin a significant reduction in the numbers of lymphocytes andmacrophages in the bronchoalveolar space. (3) When stimulatedin vitro with LPS, CCR2^-/- alveolar macrophages harvested fromeither naive mice (without transplants) or after allo-BMT producedTNF- ${alpha}$ in amounts comparable to CCR2^+/+ cells. Similar observationswere made when CCR2^-/- lymphocytes were stimulated in a mixedlymphocyte reaction (MLR).
Since previous work has identified a significant role for Th1-effectorlymphocytes in the development of IPS,^8-10 the reduction inlung injury seen after allogeneic CCR2^-/- BMT could also havebeen attributed in part to alterations in T-cell function, recruitment,or both. Our results demonstrate that the absence of CCR2 ondonor cells resulted in reduced numbers of lymphocytes in thebronchoalveolar space but had no effect on the functional capacityof these cells; lymphocytes from CCR2^-/- mice showed no deficitsin proliferation, IFN- ${gamma}$ production, or CTL activity to alloantigensboth in vitro and in vivo. It was also possible that diminishedlung injury after CCR2^-/- BMT was secondary to a Th2 shift inthe pulmonary immune response after BMT.^81,82 This was unlikelybecause lymphocytes present in the lung after CCR2^-/- BMT expressintracellular IFN- ${gamma}$ , and IL-4 was not detected in the cytoplasmof CCR2^-/- T cells or in serum or BALF of CCR2^-/- BM transplantrecipients (data not shown). Collectively, these results suggestthat impaired leukocyte recruitment rather than functional defectsin CCR2^-/- T cells and accessory cells contributed to the reductionof IPS seen after CCR2^-/- BMT.
Our studies may also shed light on the mechanism by which donorT cells contribute to the recruitment of monocytes and macrophagesduring the progression of IPS after allo-BMT. CD8⁺ T cells arethe predominant lymphocyte subset in the lungs of mice withIPS both in the P $->$ F₁ and in the B6 $->$ bm1 systems. Other studieshave shown that CD8⁺ T-cell recognition of alveolar epithelialcells triggers chemokine expression by the damaged epitheliumthat results in progressive inflammation; initial damage canbe mediated by TNF- ${alpha}$ , and subsequent leukocyte infiltration canbe abrogated by in vivo neutralization of MCP-1.^35,83-85 Inthis light, early pulmonary injury induced by infiltrating alloreactiveT cells may enhance donor monocyte and macrophage recruitmentinto the lung via enhancing local MCP-1 secretion by pulmonaryepithelial and/or endothelial cells. This possibility is supportedby our observations showing that (1) increases in MCP-1 expressioncorrelate with the initial influx of donor lymphocytes intothe lung and precede the recruitment of donor macrophages, (2)intense immunohistochemical staining of MCP-1 is found in areasof dense lymphocyte infiltration around bronchial structuresand vessels, and (3) MCP-1 neutralization coincident with theinitial recruitment of donor T cells reduces subsequent macrophageinflux and IPS severity.
In summary, our results demonstrate a critical role for CCR2/MCP-1interactions in the development of IPS. The reduction in IPSseen after allogeneic BMT with CCR2^-/- donor mice and in allogeneicwild-type (wt) recipients treated with a neutralizing antibodyto MCP-1 was dependent upon decreased recruitment of donor effectorcells into the lung. Elevated MCP-1 levels in patients withIPS suggest that CCR2/MCP-1 interactions may be operative afterclinical BMT as well. Since IPS develops and progresses to respiratoryfailure despite significant systemic immunosuppression, ourfindings suggest that novel strategies directed toward inhibitingpathways of effector cell recruitment to the lung may serveas effective adjuncts to standard therapy intended to preventor treat this serious complication.

   Footnotes

Submitted August 11, 2003; accepted November 1, 2003.
Prepublished online as Blood First Edition Paper, November 13,2003; DOI 10.1182/blood-2003-08-2708.

Supported by National Institutes of Health grants 5K12HD028820-12and RO1 HL072258-01. G.C.H. is a Deutsche Krebshilfe e.V. Scholar;K.R.C. is an Amy Strelzer-Manasevit Scholar of the NationalMarrow Program, a Fellow of the Robert Wood Johnson MedicalMinority Faculty Development Program, and the Recipient of aTranslational Research Award from the Leukemia and LymphomaSociety.

The publication costs of this article were defrayed in partby page charge payment. Therefore, and solely to indicate thisfact, this article is hereby marked "advertisement" in accordancewith 18 U.S.C. section 1734.

Reprints: Kenneth R. Cooke, University of Michigan Cancer Center, 1500 E Medical Center Dr, 6303 CCGC, Ann Arbor, MI 48109-0942; e-mail: krcooke{at}umich.edu