High numbers of tumor-infiltrating FOXP3-positive regulatory T cells are associated with improved overall survival in follicular lymphoma

doi:10.1182/blood-2006-04-018218

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Blood, 1 November 2006, Vol. 108, No. 9, pp. 2957-2964.
Prepublished online as a Blood First Edition Paper on July 6, 2006; DOI 10.1182/blood-2006-04-018218.

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CLINICAL TRIALS AND OBSERVATIONS
High numbers of tumor-infiltrating FOXP3-positive regulatory T cells are associated with improved overall survival in follicular lymphoma
Joaquim Carreras, Armando Lopez-Guillermo, Bridget C. Fox, Lluis Colomo, Antonio Martinez, Giovanna Roncador, Emili Montserrat, Elias Campo, and Alison H. Banham
From the Hematopathology Section, Departments of Pathology, and Hematology, Hospital Clinic, IDIBAPS, University of Barcelona, Barcelona, Spain; the Nuffield Department of Clinical Laboratory Sciences, University of Oxford, John Radcliffe Hospital, Headington, Oxford, United Kingdom; and Centro Nacional de Investigaciones Oncológicas (CNIO), Madrid, Spain.

   Abstract

Top
Abstract
Introduction
Patients and methods
Results
Discussion
References

The tumor microenvironment plays an important role in the biologicbehavior of follicular lymphoma (FL), but the specific cellsubsets involved in this regulation are unknown. To determinethe impact of FOXP3-positive regulatory T cells (Tregs) in theprogression and outcome of FL patients, we examined samplesfrom 97 patients at diagnosis and 37 at first relapse with ananti-FOXP3 monoclonal antibody. Tregs were quantified usingcomputerized image analysis. The median overall survival (OS)of the series was 9.9 years, and the FL International PrognosticIndex (FLIPI) was prognostically significant. The median Tregpercentage at diagnosis was 10.5%. Overall, 49 patients hadmore than 10% Tregs, 30 between 5% to 10%, and 19 less than5%, with a 5-year OS of 80%, 74%, and 50%, respectively (P =.001). Patients with very low numbers of Tregs (< 5%) presentedmore frequently with refractory disease (P = .007). The prognosticsignificance of Treg numbers was independent of the FLIPI. Seventransformed diffuse large B-cell lymphomas (DLBCLs) had lowerTreg percentages (mean: 3.3%) than FL grades 1,2 (mean: 12.1%)or 3 (mean: 9%) (P < .02). In conclusion, high Treg numberspredict improved survival of FL patients, while a marked reductionin Tregs is observed on transformation to DLBCL.

   Introduction

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Abstract
Introduction
Patients and methods
Results
Discussion
References

Follicular lymphoma (FL) is the second most common subtype ofadult B-cell non-Hodgkin lymphoma (NHL) in Western countriesand is characterized by the t(14;18) translocation. This abnormalitypromotes tumor cell survival through overexpression of the antiapoptoticBcl-2 protein. Of interest, mice overexpressing Bcl-2 underthe control of the immunoglobulin enhancer develop follicularhyperplasia rather than FL, indicating that pathogenetic mechanismsother than Bcl-2 overexpression exist in FL.¹ The vast majorityof FL patients has incurable disease with a generally indolentcourse with frequent relapses and the eventual development ofresistance to chemotherapy or transformation to an aggressivediffuse large B-cell lymphoma (DLBCL) leading to death fromdisease. Despite a common underlying genetic abnormality, theclinical course of FL patients is heterogeneous. While the mediansurvival of newly diagnosed FL patients is typically 8 to 10years, there is a significant group of patients, 10% to 15%,having a more rapid disease course that proves fatal in 2 to3 years. As yet, there is a lack of reliable prognostic markersthat can be used at the time of diagnosis to identify the high-riskpatients who will experience rapid disease progression. An internationalcooperative study has now proposed a simple and reproducibleFollicular Lymphoma International Prognostic Index (FLIPI) basedon easily available clinical data.² The parameters used to defineFLIPI represent surrogate markers of disease biology. The identificationof prognostic models more closely related to the biologic mechanismsinvolved in the development and/or progression of the tumormay provide useful information, not only to predict survivalbut also to enable the design of more targeted therapeutic strategies.
In the last few years, microarray-based gene expression profilinghas played an important role in the identification of clinicallyrelevant subtypes within B-cell lymphoma entities. Intriguingly,survival signature analysis of FL patients at the time of diagnosisgenerated 2 immune response signatures. These were based onthe molecular features of tumor-infiltrating cells and couldbe combined to effectively predict survival.³ Thus, in contrastto other B-cell lymphomas where gene expression in the malignantB-cell population determines survival, the composition of thelymphoma microenvironment at diagnosis seems to determine thesurvival of patients with FL. The immune response 1 (IR-1) signatureconferred a favorable outcome and included T-cell markers togetherwith genes highly expressed in macrophages. The immuneresponsesignature 2 (IR-2) included genes preferentially expressed inmacrophages and dendritic cells and conferred an unfavorableoutcome. However, this signature was not determined solely bythe total number of T cells since there was no correlation betweena "pan-T-signature" and survival. A recent study has confirmedthe clinical significance of macrophage numbers in FL showingthat high numbers of these cells correlated with poor survival.⁴On the contrary, further immunostaining studies in the sameFL series using a range of commonly used T-cell markers failedto identify a significant association with overall survival.⁴
A subset of regulatory T cells (Tregs), with a CD4⁺CD25⁺ immunophenotype,has recently generated considerable interest through their criticalrole in regulating immunotolerance predominantly via the suppressionof effector T-cell proliferation and cytokine production.^5-7Further studies have now convincingly identified a role forTregs in enabling tumor cells to evade the host immune response.^8-11While a number of markers (including CTLA-4, GITR, and CD45RB)are expressed on Tregs, the FOXP3 transcription factor is currentlyaccepted as the master regulator of this cell lineage and thusthe most specific Treg marker. Our production and characterizationof paraffin-reactive monoclonal antibodies to FOXP3¹² have recentlyprovided essential reagents with which to investigate the clinicalsignificance of FOXP3positive Tregs within the microenvironmentof human tumors. To determine the role of Treg immunoregulatorycells in the progression and outcome of FL, we have examineda large series of patients at diagnosis and relapse. Our resultsindicate that the number of Tregs predicts survival in FL patientsand that transformation to DLBCL is associated with a markedreduction in the number of these cells in the tumor microenvironment.

   Patients and methods

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Abstract
Introduction
Patients and methods
Results
Discussion
References

Patients and samples
Ninety-seven patients consecutively diagnosed with FL in a singleinstitution between 1988 and 2003 were included in the presentstudy, with the only criterion for inclusion being the availabilityof histologic material. All of the cases were reviewed and reclassifiedaccording to the criteria of the World Health Organization (WHO)Classification.¹³ Approval for these studies was obtained fromthe institutional review board of Hospital Clinic, Barcelona.Informed consent was provided according to the Declaration ofHelsinki. The median age of the patients was 55 years (range,26-93 years), and the male-female distribution was 49/48. Advancedstage (Ann Arbor IV) was observed in 58 cases (60%), bulky diseasein 14 (14%), and extranodal involvement in 63 (65%), includingbone marrow infiltration in 64 cases (66%). Twenty (23%) of87 patients with available data presented with high serum lacticacid dehydrogenase (LDH) levels, and 28 (38%) of 73 had highserum $beta$ 2-microglobulin ( $beta$ 2m). The distribution of the series accordingto the FLIPI² was the following: low risk, 32 cases (37%); intermediaterisk, 23 cases (27%); and high risk, 31 cases (36%). In 11 cases,FLIPI could not be calculated.
Staging maneuvers included patient history and physical examination;blood cell counts and serum biochemistry, including LDH and $beta$ 2m levels; computerized tomography scan of chest, abdomen, andpelvis; as well as unilateral bone marrow biopsy. Seventy-ninepatients were treated with combination chemotherapy (9 withCOP [cyclophosphamide, vincristine, and prednisone], 56 withCHOP-like [cyclophosphamide, adriamycin, vincristine, and prednisone]regimens, and 14 with fludarabine combinations), 7 with alkylatingmonotherapy, and 3 with radiotherapy, whereas in 8 cases a wait-and-seepolicy was established. Posttherapy restaging consisted of therepetition of the previously abnormal tests and/or biopsies.Response was assessed according to conventional criteria.¹⁴Among the 89 patients with assessable response, 58% of the patientsachieved a complete response (CR) and 33% a partial response,whereas 9% failed to respond to treatment. After a median follow-upof 5.6 years (range, 1.1-13.0 years) for surviving patients,33 patients had died. The 5-year and 10-year overall survival[OS] was 72% (95% confidence interval [CI]: 62%-82%) and 52%(95% CI: 38%-66%), respectively.
In addition to the diagnostic tissue samples, sequential specimensat relapse were available for 18 patients. These were used toassess the numbers of FOXP3-positive Tregs over time. Finally,samples at relapse from another 19 patients from the same institution,for whom no additional material from the diagnostic biopsy wasavailable, were also examined. All 37 samples were used to studythe clinicopathological significance of FOXP3-positive Tregsat relapse in FL.
Finally, numbers of FOXP3-positive Tregs were analyzed in 6reactive tonsils, in order to examine their frequency and distributionin normal lymphoid tissue.
Immunohistochemistry
Tissue samples were fixed in formalin and embedded in paraffinby routine methods. Immunostaining was performed in one laboratory(B.C.F. and A.H.B.) using undiluted hybridoma supernatant ofthe 236A/E7 anti-FOXP3 murine monoclonal antibody.¹² Sectionswere dewaxed in Citro-clear (HD Supplies, Aylesbury, UnitedKingdom), and antigen retrieval was performed by microwave pressurecooking for 11 minutes in 50 mM Tris, 2 mM EDTA, pH 9. Serialsections were also stained for CD3 and CD4 (anti-CD3 monoclonalantibody, clone SP1, dilution 1:60; anti-CD4 monoclonal antibody,clone 4B12, dilution: 1:10; Novocastra, Newcastle upon Tyne,United Kingdom). Detection was performed using the EnVision-system(DakoCytomation, Glostrup, Denmark) according to the manufacturer'sinstructions. Tonsil sections were immunolabeled in parallelas a positive control together with the isotype-matched MR12antibody as a negative control.
Quantitative assessment of FOXP3-positive Tregs, and CD3⁺ and CD4⁺ cells
The number of FOXP3-positive Tregs was quantified in whole-tissuesections of all samples using an automated scanning microscopeand image analysis system (Ariol 2.1, SL-50; Applied Imaging,Melville, NY). Quantification of the FOXP3-positive cells wasperformed with the nuclear Kisight Assay provided by the manufacturer(Applied Imaging), using the following strategy. First, thetissue find phase was performed at 1x objective followed byan automated low-magnification scanning with the 5x objective.Subsequently, the optimal evaluation areas, which accountedfor 60% to 100% of the whole section, were selected by the observer(J.C.) and scanned at high magnification with the 20x objective.In the next review phase, a nuclear high-resolution classifierwas created and trained for the FOXP3 nuclear staining. Theclassifier consisted of a color class definition for the positiveand negative nuclei and background, and a shape class definitionfor the positive and negative nuclei. The color class was definedby the hue, saturation, and intensity parameters, whereas theshape class was defined by the spot width, width, compactness,roundness, and axis ratio parameters. The FOXP3 high-resolutionclassifier was trained in several areas within a tissue samplein order to avoid miscalculation due to differences in stainingand cell composition. Among tissue samples, the classifier wasalways trained and recalibrated under the visual supervisionof the pathologist. FOXP3-positive and -negative cells werecounted independently in the follicular and interfollicularcompartments. The follicular compartment included the mantlezone when present. The total number of cells was recorded byadding the counts for the 2 compartments. To minimize the heterogeneousdistribution of positive cells, a minimum number of 6 completefollicular and interfollicular areas was selected in tumorswith a predominantly nodular pattern. In tumors with a predominantlydiffuse pattern, a minimum of 6 high-power fields (HPFs) wasevaluated. The selected areas had a similar number of totalcells and were representative of the overall distribution ofFOXP3-positive Tregs, and tangential sections of follicles wereavoided. In areas in which the images of the nuclei were fusedforming a net pattern, shape classes were established in clearlyidentifiable individual cells and the settings applied to therest of the sample. In tumors with diffuse and nodular patterns,these areas were quantified and recorded separately. The meannumber of total counted cells per case was 34 840 (range, 4754-169330) corresponding to 21.2 HPFs (range, 3-103 HPFs; mean celldensity, 1644 cells/HPF) (UplanFI 40x/0.75; Olympus). Once areaswere selected by the observer, the software collected the dataautomatically. The observer (J.C.) was blinded to the clinicaldata of the patient.
The number of CD3⁺ and CD4⁺ cells was also quantified with thesame methodology in whole tissue sections of all samples, usingthe same automated scanning microscope and image analysis system.Since the staining was cytoplasmic and membranous, we used theGensight Multistain Assay also provided by the manufacturer(Applied Imaging) and only the color class parameters were trained.
Statistical analysis
The main initial and evolutive variables, including the histologicparameters, were recorded and analyzed for the prognostic significance.Categoric data were compared using Fisher exact test, 2-sidedP value, whereas for ordinal data nonparametric tests were used.The multivariate analysis of the variables predicting responsewas performed by using a logistic regression. The actuarialsurvival analysis was performed according to the method describedby Kaplan and Meier, and the curves were compared by the log-ranktest. The independent prognostic value of FOXP3-positive Tregnumbers and clinical data summarized in the FLIPI was testedby means of the stepwise proportional hazards model of Cox.
Images in Figures 1 and 2 were acquired using an Olympus BX51clinical microscope and DP70 digital camera and software (Olympus,Tokyo, Japan). Original magnification, x200 (objective lens,UPlanApo 20 /0.70 NA).

   Results

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Abstract
Introduction
Patients and methods
Results
Discussion
References

Clinical and histologic characteristics of patients at diagnosis
The main clinical and histologic features of the 97 patientsat diagnosis are detailed in "Patients, materials, and methods"and summarized in Table 1. The histologic distribution accordingto the WHO classification was grade 1, 24 cases (25%); grade2, 57 cases (58%); and grade 3, 16 cases (17%) (grade 3a, 12cases [12%], grade 3b, 4 cases [4%]). The architectural patternwas predominantly follicular (follicular area > 75%) in 83cases (86%), follicular and diffuse (follicular area 25%-75%)in 5 (5%), and predominantly diffuse (follicular area < 25%)in 9 (9%) cases. Two cases, one grade 1 and one grade 3 FL,had a small component of diffuse large B-cell lymphoma in thesame lymph node biopsy at diagnosis.

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Table 1.. Main clinical and histopathologic features of 97 patients with FL at diagnosis

FOXP3-positive Tregs in FL at diagnosis
FOXP3-positive Tregs were observed in all cases, but the numberand topographic distribution within the tumor varied from caseto case. The distribution of the positive cells could be categorizedinto 4 major immunohistochemical patterns: interfollicular,follicular, perifollicular/mantle zone, and mixed perifollicularand interfollicular (Figure 1). In the interfollicular pattern,most of the Tregs were observed between the follicles (Figure 1A),whereas in the follicular pattern there were more Tregs withinthe follicles than in the interfollicular areas (Figure 1B).The perifollicular/mantle zone pattern was characterized bya prominent infiltration of Tregs surrounding the nodules (Figure 1C).Finally, some cases had a mixed pattern with strong infiltrationin the perifollicular area and in the interfollicular spaces(Figure 1D). The distribution of the patients according to thesepatterns was as follows: follicular, 5 patients (5%), perifollicular/mantlezone, 13 (13%), interfollicular, 60 (62%), and mixed, 10 (10%).Nine patients had a predominantly diffuse architectural pattern,and in these cases Tregs were scattered throughout the tumor.These visual immunohistochemical patterns did not show any significantcorrelation with the clinical and histopathologic features ofthe patients.
To determine whether the total number of Tregs infiltratingthe tumor could have a specific relationship with the clinicopathologicalcharacteristics of the patients, we quantified the number ofFOXP3-positive Tregs using a computerized image analysis systemwith an automated scanning microscope. The cells were quantifiedseparately in the interfollicular and in the follicular compartments.The total number of Tregs was calculated by adding these 2 counts.The mean number of total counted cells per case was 34 840 (range,4754-169 330). The median percentage of Tregs in the 97 diagnosticbiopsies was 10.5% (range, 0.9%-42.5%). Overall, 49 patients(50%) had a Treg count of more than 10%, 30 (31%) between 5%to 10%, and 18 (19%) less than 5%.
The relationship between the number of Tregs in samples at diagnosisand the pathological characteristics of the patients is shownin Table 2. The numbers of Tregs were lower in the follicularthan in the interfollicular compartment (mean ± SD: 8.6%± 5.2% vs 14.7% ± 9.7% for follicular and interfollicularareas, respectively; P < .001). Grade 3 FL had lower numbersof Tregs than grades 1 or 2 when the follicular compartmentwas assessed (6.7% vs 9%; P = .048) (Table 2).

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Table 2.. Distribution of FOXP3-positive Tregs in 97 FL at diagnosis

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Figure 1.. Immunohistochemical FOXP3-positive Treg patterns. (A) Interfollicular pattern. (B) Follicular pattern. (C) Perifollicular pattern. (D) Mixed pattern.

Tumors with a predominantly diffuse pattern showed a lower numberof Tregs (9.3%) than cases with a predominantly follicular pattern(11.8%), although this difference was not statistically significant.Of interest, in 5 FLs with mixed follicular and diffuse patternat diagnosis, the number of Tregs in the diffuse component wassignificantly lower than in the follicular areas (8.03% vs 13.1%;P = .043) (Table 3). Similarly, in 2 patients that presentedat diagnosis with a DLBCL component, the number of Tregs inthese DLBCL areas (1.02%) was lower than in the FL areas (6.9%)of the same biopsy (Table 4).

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Table 3.. Distribution of FOXP3-positive cells in 5 grade 2 FLs, nodular and diffuse at diagnosis

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Table 4.. Distribution of FOXP3-positive cells in 2 FL/DLBCL at diagnosis

Finally, FOXP3-positive Tregs were also evaluated in 6 reactivetonsils. The percentage of total Tregs in these samples was9.5% ± 5.9%, whereas the FL samples contained 11.6% ±7.5% (P > .1). The number of Tregs in the follicular andinterfollicular compartments was also counted separately. Ofinterest, the number of Tregs in the follicular compartmentof FL was higher than in reactive tonsils (8.6% ± 5.6%vs 3.7% ± 1.9%; P = .012). Conversely, no differencesbetween the FL and reactive tonsils were found when analyzingthe interfollicular compartment (13.3% ± 10.2% vs 12.6%± 7.7%).
Relationship between FOXP3-positive Treg numbers, clinical features, and outcome
Treg numbers were compared with the main clinical features ofthe patients at diagnosis (Table 5). No significant correlationwas observed between the Treg number and the main initial characteristics,including Ann Arbor stage, nodal and extranodal involvement,serum LDH, or serum $beta$ 2-microglobulin. However, patients withhigh-risk FLIPI more frequently exhibited a Treg count of lessthan 10% than did those with low- or intermediate-risk FLIPI(74% vs 44%, respectively; P = .007).

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Table 5.. Correlation between main clinicohistologic features and overall FOXP3-positive Treg number in diagnostic samples

There were no differences in the treatment given to the patientson the basis of the number of Tregs. Regarding the responseto therapy, those patients with a very low number of Tregs (<5%) presented more frequently with refractory disease (failureto first-line treatment) than the others (5 [30%] of 15 vs 4[6%] of 70, respectively; P = .007). No significant differenceswere found in terms of event-free survival according to theTreg number.
Median overall survival (OS) of the series was 9.9 years, andthe OS curve is plotted in Figure 3A. The main clinicobiologicvariables with favorable impact on OS were the following: ageyounger than 60 years; ambulatory performance status (ECOG <2); absence of B symptoms; number of nodal sites less than 4;and normal hemoglobin level, serum LDH, $beta$ 2m, and histologic grade(grade 1 and 2 vs 3). FLIPI score divided the series into 3groups of low, intermediate, and high risk with median OS of3.9 years, 9.3 years, and not reached, respectively (Figure 3B).OS according to the Treg number is plotted in Figure 4. Five-yearOS of patients with Tregs less than 5%, 5% to 10%, and morethan 10% was of 50% (95% CI: 26%-74%), 74% (95% CI: 54%-94%),and 80% (95% CI: 68%-92%), respectively (P = .001) (Figure 4A).Moreover, the quantity of Tregs in the follicular compartmentalso showed prognostic value for OS, with a 5-year OS of 79%,76%, and 61% for Tregs more than 10%, 5% to 10%, and less than5%, respectively (P = .02) (Figure 4B). In contrast, interfollicularTreg numbers were not predictive of patient outcome.
To determine whether the prognostic significance of FOXP3-positiveTregs was only a surrogate marker of the number of CD3⁺ T cells,80 FL samples at diagnosis were stained and quantified for CD3.Although the number of Tregs showed a correlation with the numberof CD3⁺ cells when analyzed as a categoric variable (CD3 percentagemedian: 30% vs 49% for cases with CD3⁺ cells below and abovethe Treg median, respectively; P = .001), the ratio was notsignificant in a linear regression test (R square = 0.092).The number of CD3⁺ cells counted in the whole section separatedin 3 groups did not show predictive significance for OS. Five-yearOS of patients with CD3 less than 30%, 30% to 50%, and morethan 50% was 72% (95% CI: 54%-90%), 63% (95% CI: 39%-87%), and87% (95% CI: 73%-100%), respectively (P = .15) (Figure 5A).The same study carried out in the follicular and interfollicularcompartments did not show predictive value for OS.

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Figure 2.. Tregs in FL and DLBCL. (A) FL at diagnosis. (B) The lymph node biopsy of the same patient at relapse shows a transformed DLBCL with a lower number of Tregs.

Moreover, to determine whether the prognostic significance ofFOXP3-positive Tregs was only a surrogate of the number of CD4⁺T cells, 71 FL samples at diagnosis were stained and quantifiedfor CD4 as well. The total number of CD4⁺ cells did not showa correlation with the number of Tregs either when analyzedas a categoric variable (median CD4: 41 vs 40 for cases belowand above Treg median, respectively; P = .8) or in the linearregression test (R square: 0.007). In addition, CD4⁺ cells didnot have prognostic value for OS (5-year OS of patients withCD4 < 31%, 31%-46%, and > 46% was 69% [95% CI: 48%-90%],74% [95% CI: 54%-94%], and 58% [95% CI: 35%-81%], respectively;P = .7) (Figure 5B). The same negative result was observed whenthe analysis was performed in the follicular and the interfollicularcompartments. Of note, in these sets of patients, the numberof FOXP3-positive Tregs maintained its predictive value forOS.
To further analyze the prognostic importance of the number ofTregs, a Cox analysis was performed, including Treg number ( $≤$ 10% vs > 10%) and FLIPI score (low, intermediate, and high).In the final model, with 86 assessable cases, Treg number maintainedits predictive value (relative risk: 0.59 [95% CI: 0.34-0.84];P = .04) along with the FLIPI (relative risk: 2.7 [95% CI: 2.47-2.94];P < .001). However, when the histologic grade (grade 1,2vs grade 3) was also included in the analysis, only FLIPI andhistologic grade showed prognostic significance, whereas theTreg number had only marginal value.

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Figure 3.. Overall survival of the study population. (A) Overall survival of 97 patients with FL. (B) Overall survival according to the FLIPI score (P = .003).

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Figure 4.. Overall survival in patients with FL in relation to FOXP3-positive Tregs. (A) Overall survival according to FOXP3-positive Tregs (P < .05). (B) Overall survival according to follicular FOXP3-positive Tregs (P < .05).

FOXP3-positive Tregs in FL at first relapse
A sample obtained at the first relapse after the diagnosis ofFL was available from 37 patients. The histologic distributionof these biopsies at relapse was FL grade 1, 5 cases (14%);grade 2, 20 cases (54%); grade 3, 7 cases (18%); and transformationto a DLBCL, 5 (14%) cases. After excluding the DLBCL cases,24 FL cases (75%) had a predominantly nodular pattern and 8cases (25%) a predominantly diffuse pattern.

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Figure 5.. Overall survival in patients with FL in relation to CD3⁺ and CD4⁺ cells. (A) Overall survival according to CD3⁺ cells (P = NS). (B) Overall survival according to CD4⁺ cells (P = NS).

The mean of Tregs in the relapsed samples was 8.7%. Similarto samples at diagnosis, the number of Tregs was lower in thefollicular than in the interfollicular compartment (8.4% vs14.3%; P = .001), and the diffuse areas tended to have fewerTregs than the follicular areas (7.6% vs 10.6%, P = .063). Ofinterest, the DLBCL had a significant decrease in mean Tregnumbers (2.2%) compared with the FL grades 1 and 2 (9.6%) and3 (10.5%) (P = .006). The low numbers of Treg in these DLBCLsat relapse was similar to the number of Tregs in the DLBCL componentdetected in 2 FLs at diagnosis.
Sequential samples at diagnosis and at first relapse were availablefor 18 patients. Twelve cases maintained the same FL grade inboth samples, 2 cases progressed from an FL grade 1 and 2 toan FL grade 3, 1 case showed a downgrading from an FL grade3 to an FL grade 1, and 3 cases transformed from an FL grade2 (1 case) or FL grade 3 (2 cases) to a DLBCL (Table 6). Thenumber of Tregs was similar at diagnosis and at relapse in thecases with either no modification of the tumor grade or downgrading,but decreased in both the progressed grade 3 FL (mean: 18.7%vs 15.1%) and in the transformed DLBCL cases (mean: 15.5% vs4.9%) (Table 6). The median survival from the first relapsewas 4.4 years. No significant correlation was found betweenTreg number (both total and follicular) and survival from relapse.

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Table 6.. Distribution of FOXP3-positive Treg in 18 FL with sequential samples at diagnosis and first relapse

Overall, in this study we have examined 7 transformed DLBCLs,2 observed at diagnosis concomitantly with FL (one with grade1 and one with grade 3) and 5 at first relapse. The total numberof infiltrating Tregs in these tumors was significantly lower(mean: 3.3%) than in the FL at diagnosis (grade 1 and 2, mean:12.1%; grade 3, mean: 9%) or at first relapse (grade 1 and 2,mean: 9.6%; grade 3, mean: 10.5%) (P < .02) (Figure 2).

   Discussion

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Abstract
Introduction
Patients and methods
Results
Discussion
References

The tumor cell microenvironment is now thought to play a criticalrole in the biology of a number of B-cell lymphomas.^15-18 Severalstudies have indicated the important influence of tumor cellmicroenvironment in the pathogenesis of FL. First, these tumorcells are difficult to grow in vitro unless they are stimulatedwith stromal cells and a combination of CD40 and cytokine signals¹⁹or cocultured with CD4 T cells recognizing lymphoma alloantigens.²⁰Another important observation is the ability of patients withFL to undergo spontaneous tumor regression, highlighting therole of immunosurveillance mechanisms in this disease.²¹
Gene expression studies of FL have also emphasized the impactof immunoregulatory cells on the clinical behavior and responseto therapy of these tumors.^3,22-24 In particular, an expressionsignature characterized by a combination of genes mainly expressedby T cells and macrophages has been associated with good prognosis,whereas an expression signature composed of genes highly expressedin macrophages and dendritic cells has been correlated withshorter survival.³ Although the microarray studies suggest thatthe relationship between the macrophage/dendritic cell populationand prognosis may be complex, a recent immunohistochemical studyhas confirmed the impact of the total number of macrophagesin the aggressive clinical evolution of FL.⁴ The T-cell population(s)that may influence the behavior of FL tumor cells is not clear.The microarray studies indicated that the T-cell signature associatedwith good prognosis was not a direct consequence of the totalnumber of tumor-infiltrating T cells.³ Similarly, the immunohistochemicaldetection of the most common T-cell–associated markersdid not reveal any particular subpopulation of cells relatedto survival in FL.⁴
In the present study, we demonstrate that the number of tumorinfiltratingFOXP3-positive Tregs is a predictor of survival in patientswith FL, independently of the FLIPI, and that the number ofthese cells decreases during the transformation to DLBCL. Incommon with other studies,^3,4 total T-cell numbers had no prognosticsignificance in this series. These results suggest that Tregsmay be an important subset of cells in the tumor microenvironmentmodulating the host immune response and biologic behavior ofFL. Tregs are a subpopulation of T lymphocytes that play a crucialrole in the control of T-cell–mediated autoimmunity bysuppressing the proliferation and cytokine production of otherT cells.^5,25,26 These cells seem also to participate in theregulation of the immune response against tumor cells, representingan important element of the cancer microenvironment. Thus Tregsmay suppress tumor-specific T-cell immunity, thereby contributingto cancer cell growth.⁹ Concordantly, the presence of a highnumber of these cells in the solid tumors has been correlatedwith a poor prognosis of patients.^9,11,27 However, most of thesestudies have been performed on carcinomas, with the role ofTregs in hematologic malignancies being less established. Arecent study in patients with B-CLL identified the highest numbersof CD4⁺CD25⁺ Tregs in untreated or progressing patients presentingwith extended disease, and both numbers and suppressive functionwere decreased on treatment with fludarabine.²⁸ However, thisstudy in B-CLL investigated Treg numbers only in the peripheralblood. Contrary to these observations, we report here that FLpatients with higher Treg numbers in their tumors had a betterresponse to therapy and improved overall survival. In this seriesof FL patients, the FLIPI effectively segregated the patientsinto prognostically relevant groups. Of interest, the prognosticvalue of the number of Tregs was independent of the FLIPI score,suggesting that this parameter reflects a different biologicaspect of the tumors. These data are similar to previous findingsin Hodgkin lymphoma, where a high number of FOXP3-positive Tregswas also associated with improved patient survival.²⁹ Takentogether, these studies suggest that the role of Tregs in thepathogenesis of these B-cell lymphomas is different than incarcinomas.
A recent study has shown that Treg numbers are increased inB-cell non-Hodgkin lymphoma tissues compared with reactive tonsilor lymph nodes, probably being recruited via CCL22 secretedby the malignant B cells. Of importance, these intratumoralFOXP3-positive Tregs from lymphoma patients were demonstratedto be functionally capable of suppressing the proliferationand cytokine production of CD4⁺ T cells.⁷
Generally, the suppressive activity of CD4⁺CD25⁺ Tregs is dependenton T-cell receptor activation or T-cell priming. T-cell receptoractivation could regulate not only the effector function ofTregs but also their migratory behavior. Thus, upon T-cell activation,Tregs may migrate from the T-cell–rich zone to the germinalcenters by switching the chemokine receptor CCR7 expressed bythe interfollicular Tregs to the CXCR5, the specific receptorfor the follicle-homing chemokine CXCL13.³⁰ Of interest, intrafollicularTregs suppress germinal center T helper (GC-Th) cells and theGC-T–induced B-cell responses such as immunoglobulin (Ig)production and expression of activation-induced cytosine deaminase(AID).³⁰ In addition, GC-Tregs also suppress the GC-Th–cell–dependentsurvival of B cells.³⁰ Moreover, Tregs may have a direct effecton B cells.^30-32 Thus, a recent report has described that, underT-cell–free activation conditions, FOXP3-positive Tregsare able to directly suppress B cells by reducing the expressionof AID and inhibiting their Ig class switch recombination andIg production.³² Besides, Tregs may suppress B-cell proliferationby inducing cell death mediated by a cytotoxic-dependent pathway.³³All these observations on the specific direct and indirect B-cellinhibitory functions of the GC-Tregs allow us to hypothesizethat the favorable clinical impact of a high number of Tregsin FL patients may be due to their inhibitory effects on thetumor cells. In this sense, it is interesting that in our studythe number of Tregs in the follicular compartment, but not inthe interfollicular area, was a predictor of a better outcomein patients.
The natural history of FL is characterized by continuous relapsesthat become progressively less sensitive to chemotherapy.³⁴The analysis of prognostic factors at relapse should be usefulto select patients for whom inclusion in experimental trialsis warranted. Several clinical parameters, including responseduration and FLIPI among others, seem to be of prognostic significancein FL at first relapse.^34-36 However, the predictive significanceof biologic markers at relapse in FL has not been well examined.In this study, we have assessed the prognostic value of Tregnumbers in FL at first relapse. Contrary to the results in thesamples at diagnosis, the number of Tregs at first relapse didnot predict survival. However, the number of patients was relativelylow to draw definitive conclusions. Of interest, we could examinesequential samples in 18 patients obtained at diagnosis andfirst relapse. The Treg infiltrate was similar in tumors thatrelapsed with the same cytologic grade and decreased slightlyin tumor progressing from grade 1 or 2 to grade 3. However,the number of these cells was dramatically reduced in casesthat transformed to DLBCL. These extremely low numbers of Tregswere also observed in the 2 DLBCL components present at diagnosisand in 2 additional cases diagnosed at the first relapse inwhich the biopsy at diagnosis could not be examined. These observationsindicate that transformation of FL to DLBCL is associated witha marked reduction in the Treg infiltrate. Although the lownumbers of Tregs may facilitate the progression of the tumorsby releasing inhibitory signals upon the tumor B cells, furtherstudies are needed to determine the potential role of thesecells in the progression of FL.
In summary, the results of this study show that high numbersof Tregs are not related to the total numbers of CD3⁺ and CD4⁺cells and predict improved overall survival in FL independentlyof the FLIPI. In addition, transformation to DLBCL is associatedwith a marked reduction in the number of associated Tregs, suggestingthat these cells may also play a role in tumor progression.These findings support the idea that tumor-infiltrating Tregsmay be an important subset of cells modulating the tumor microenvironmentand influencing the biologic behavior of FL. A better understandingof the biologic role of FOXP3-positive Tregs in these tumorsshould assist in the development of therapeutic strategies basedon the immunomodulation of the tumor microenvironment.

   Footnotes

Submitted April 20, 2006; accepted June 20, 2006.
Prepublished online as Blood First Edition Paper, July 6, 2006;DOI 10.1182/blood-2006-04-018218.

E.C. and A.H.B. contributed equally to the study.

Supported by the Spanish Ministry of Education and Science (SAF05/5855), Instituto de Salud Carlos III, Redes Temáticasde Investigación Centros de Cáncer (C03/10) andRed de Estudio de Linfomas (G03/179), and the Leukaemia ResearchFund.

J.C. was responsible for producing the database, histopathologicrevision of the samples, quantifying the immune marker, dataanalysis, and preparing the final manuscript; A.L.-G. was responsiblefor acquiring of clinical data and the statistical analyses;B.C.F. performed the immunohistochemical staining; L.C. wasresponsible for the histopathologic revision of the samples,data acquiring, and data analysis; A.M. contributed to the dataanalysis; G.R. produced and characterized the anti-FOXP3 monoclonalantibody; E.M. was responsible for evaluating the clinical data;and E.C. and A.H.B. contributed to the design of the project,data analysis, and writing of the paper. All authors reviewedand approved the final version.

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: Elias Campo, Department of Pathology Hospital Clinic, University of Barcelona, Villarroel 170, 08036-Barcelona, Spain; e-mail: ecampo{at}clinic.ub.es.

   References

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Abstract
Introduction
Patients and methods
Results
Discussion
References

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  Copyright © 2006 by American Society of Hematology         Online ISSN: 1528-0020





	Copyright © 2006 by American Society of Hematology Online ISSN: 1528-0020