24 Feb 2010: Sweiss NJ, Salloum R, Gandhi S, Alegre ML, Sawaqed R, et al. (2010) Correction: Significant CD4, CD8, and CD19 Lymphopenia in Peripheral Blood of Sarcoidosis Patients Correlates with Severe Disease Manifestations. PLOS ONE 5(2): 10.1371/annotation/a75007e1-492a-4bcb-80a8-28b4d432c099. https://doi.org/10.1371/annotation/a75007e1-492a-4bcb-80a8-28b4d432c099 View correction
Sarcoidosis is a poorly understood chronic inflammatory condition. Infiltration of affected organs by lymphocytes is characteristic of sarcoidosis, however previous reports suggest that circulating lymphocyte counts are low in some patients with the disease. The goal of this study was to evaluate lymphocyte subsets in peripheral blood in a cohort of sarcoidosis patients to determine the prevalence, severity, and clinical features associated with lymphopenia in major lymphocyte subsets.
Lymphocyte subsets in 28 sarcoid patients were analyzed using flow cytometry to determine the percentage of CD4, CD8, and CD19 positive cells. Greater than 50% of patients had abnormally low CD4, CD8, or CD19 counts (p<4×10−10). Lymphopenia was profound in some cases, and five of the patients had absolute CD4 counts below 200. CD4, CD8, and CD19 lymphocyte subset counts were significantly correlated (Spearman's rho 0.57, p = 0.0017), and 10 patients had low counts in all three subsets. Patients with severe organ system involvement including neurologic, cardiac, ocular, and advanced pulmonary disease had lower lymphocyte subset counts as a group than those patients with less severe manifestations (CD4 p = 0.0043, CD8 p = 0.026, CD19 p = 0.033). No significant relationships were observed between various medical therapies and lymphocyte counts, and lymphopenia was present in patients who were not receiving any medical therapy.
Citation: Sweiss NJ, Salloum R, Ghandi S, Alegre M-L, Sawaqed R, Badaracco M, et al. (2010) Significant CD4, CD8, and CD19 Lymphopenia in Peripheral Blood of Sarcoidosis Patients Correlates with Severe Disease Manifestations. PLoS ONE 5(2): e9088. https://doi.org/10.1371/journal.pone.0009088
Editor: Jacques Zimmer, Centre de Recherche Public de la Santé (CRP-Santé), Luxembourg
Received: December 29, 2009; Accepted: January 20, 2010; Published: February 5, 2010
Copyright: © 2010 Sweiss et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
Funding: Grant Support and Disclosures: TB Niewold: NIH K08 AI083790, NIAID Clinical Research Loan Repayment AI071651, Arthritis National Research Foundation Eng Tan Scholar Award, Lupus Research Institute, University of Chicago CTSA Core Subsidy Grant and Collaborative University of Chicago/Northshore University Health System Translational Research Pilot Grant from UL1 RR024999. NJ Sweiss: Investigator initiated grant support from Abbott, Genentech and BMS for sarcoidosis research, Young investigator award, Foundation for Sarcoidosis Research. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Competing interests: The commercial funders, BMS, Genentech and Abbott, supported clinical trial research in sarcoidosis to use novel therapies. It did not support the work in this manuscript and does not alter adherence to PloS One polices. The authors have no financial conflicts of interest.
Sarcoidosis is a systemic inflammatory disease characterized by noncaseating granulomas which consist of CD4+ T-cells and macrophages surrounded by CD8+ T-cells . This inflammation can affect any number of organs, including the lung, liver, heart, skin, and nervous system. The etiology of sarcoidosis is unknown, but likely involves genetic factors, which interact with environmental exposures to result in disease susceptibility . The immune dysregulation in sarcoidosis is classically manifested by hypergammaglobulinemia and paradoxical cutaneous anergy to particular antigens such as tuberculin protein . This paradox of anergy co-existing with an inflammatory condition remains poorly understood.
Lymphopenia occurs in over 50% of sarcoidosis patients and is associated with chronic disease , , . While early studies have suggested that sarcoidosis-associated lymphopenia is due to T-cell depletion , few studies have focused on the various peripheral blood lymphocyte subsets in sarcoidosis. Miyara and colleagues investigated the presence and function of regulatory T cells in the lung and blood of patients with sarcoidosis. It was demonstrated that CD4+CD25brightFoxP3+ cells accumulated in the periphery of sarcoid granulomas, in BAL washings, and in peripheral blood of patients with active disease. These cells effectively suppressed the proliferation of effector cells but not their production of TNF. This may explain the paradoxical state of T cell anergy in these patients that is associated with active local inflammation. However, to our knowledge, detailed examination of the various lymphocyte subsets in the peripheral blood in sarcoidosis patients has not been described. Thus, the goal of this study was to evaluate lymphocyte subsets in peripheral blood in a cohort of sarcoidosis patients followed at the University of Chicago Rheumatology Clinic to determine the prevalence, severity, and clinical features associated with lymphopenia in major lymphocyte subsets.
Materials and Methods
We performed a retrospective review of the laboratory records for lymphocyte subset testing in sarcoidosis patients at the University of Chicago Hospital between November 2006 and January 2008. Our analysis was limited to individuals who received full testing by flow cytometry and included the following cell counts: Absolute CD4 (515–1642 cells/µL), CD8(212–887 cells/µL) and CD19 (103–581 cells/µL). The medical records of patients and controls were reviewed according to the study approved by the University of Chicago Institutional Review Board. Because this was a retrospective chart review, patient consent was waived by the Institutional Review Board as the study approved by the Institutional Review Board required no therapeutic intervention. Twenty-eight patients were identified. Inclusion criteria were patients with biopsy-proven sarcoidosis who attended the University of Chicago Sarcoidosis Center for new or return appointments and had full lymphocyte subset data available.
Clinical data were obtained by the primary study physician (NJS) and abstracted to include clinical manifestations related to sarcoidosis, demographics, and medical therapy. Lymphocyte subset data in the sarcoidosis cohort were compared to 100 healthy individuals who were tested by the clinical laboratory for assay standardization. Results were also compared between groups of patients defined by disease manifestations or medical treatment. Severe organ system involvement was defined as chronic sarcoidosis with at least one of the following disease manifestations: neurologic, cardiac, ocular, or advanced pulmonary disease defined as forced vital capacity (FVC)<40% of predicted. Patients with severe sarcoidosis typically require corticosteroid-sparing agents secondary to corticosteroid failure.
CD4, CD8, and CD19 cells were counted in whole blood using flow cytometry techniques at the University of Chicago Clinical Laboratory following standard protocols with fluorescently labeled antibodies. The proportion of cells positive for CD4, CD8, and CD19 was multiplied by the total number of lymphocytes, and cell counts were reported as number of cells per microliter (cells/µL). Normal ranges for CD4, CD8, and CD19 cell populations were derived from the healthy donor cohort used to standardize the assay. Low count was defined as results below the lower level of normal for CD4 (515–1642 cells/µL), CD8 (212–887 cells/µL) and CD19 (103–581 cells/µL).
Fisher's exact test was used to compare categorical data, and quantitative comparisons were performed using an unpaired t-test or Mann-Whitney non-parametric t-test as appropriate depending upon whether the data were normally distributed as assessed by the D'Agostino and Pearson omnibus normality test. P-values shown are all two-sided, and uncorrected for multiple comparisons.
In this cohort of 28 sarcoidosis patients, 18 were African-American, and ten were European-American. The mean age was 51.6 years, with a wide spectrum of organ system involvement (Table 1). Seven patients (25%) had cardiac and 7 had skin involvement, 4 patients (14%) had clinically significant lung involvement, 4 (14%) had neurologic involvement, and 6 patients (21%) had liver involvement. A total of 24/28 patients in this cohort (86%) required therapy.
Significant CD4, CD8, and CD19 Lymphopenia Was Present in Sarcoidosis Patients
The majority of sarcoidosis patients exhibited reduced lymphocyte subset counts, including CD4 (57%), CD8 (54%), and CD19 cell counts (54%) as compared to healthy controls (Figure 1A, p<4×10−10). Only eight patients (29%) demonstrated values within the normal range for all three lymphocyte subsets. Lymphopenia was profound in some cases, and five of the patients had absolute CD4 counts below 200. There were no significant differences by gender or ethnicity (European vs. African-American ancestry) in any of the lymphocyte subset counts. CD4, CD8, and CD19 lymphocyte counts were significantly correlated (Spearman's rho 0.57, p = 0.0017, Figure 1B), and 10 patients (36%) exhibited reduced lymphocyte counts in all three subsets.
A) Peripheral blood lymphocyte measurements show that 16 patients (57%) had lower than normal CD4 counts, 15 patients (54%) had lower than normal CD8 counts, and 15 patients (54%) had lower than normal CD19 counts. The box indicates the normal range for cell counts (95% of normal control subjects fell within this normal range) (p<4×10−10). B) Correlation between lymphocyte counts in sarcoidosis patients. CD4∶CD8 correlation shown in purple, and CD4∶CD19 shown in blue, with Spearman's rho and p-value indicated for each correlation.
Lymphopenia in Sarcoidosis Patients Is Not Related to Medical Therapy but Instead to Severity of Disease
Reductions in lymphocyte subset counts were not significantly different in patients who were taking disease-modifying anti-rheumatic drugs (DMARDs, including methotrexate, azathioprine, leflunomide and mycophenolate mofetil) (n = 14), prednisone (n = 18) or tumor necrosis factor alpha (TNF-α) inhibitors (n = 6) (p>0.5, data not shown). Four patients had not been taking any medical therapy, and three of these patients had abnormally low lymphocyte counts. Patients with severe organ system involvement as defined in the Methods had lower lymphocyte subset counts as a group than those patients who did not have these disease manifestations (CD4 p = 0.0043, CD8 p = 0.026, CD19 p = 0.033, Figure 2).
This study provides the first report of frequent and severe CD4, CD8, and CD19 lymphopenia in sarcoidosis patients to our knowledge. All lymphocyte subsets were highly correlated with each other, suggesting that many patients have severe overall T- and B-cell lymphopenia in peripheral blood. Lymphopenia was frequently present in patients who were not receiving any medical therapy, and while immunosuppressive therapies may reduce lymphocyte numbers in the peripheral blood , we found that there were no significant relationships between specific medical therapies and lymphocyte counts. In contrast, severe organ system involvement was associated with lower lymphocyte subset counts, suggesting that lymphopenia may relate more to disease pathology than medical therapy. This finding could suggest that lymphocytes are depleted in peripheral blood due to increased infiltration of target organs. In one study of pulmonary sarcoidosis patients undergoing bronchoalveolar lavage (BAL), there was a was a significant relationship between an increase in the number of CD4 positive T cells in the BAL fluid and a decrease in the absolute number of CD4 positive T cells in the peripheral blood . Alternatively, lymphopenia could represent either suppression of lymphogenesis due to cytokines or other influences, or increased peripheral destruction due to activation-driven cell death or other mechanisms. Longitudinal follow up studies would be of high interest to determine whether lymphopenia is corrected with therapy, as other disease manifestations are effectively treated. Such results would further strengthen the hypothesis that lymphopenia underlies disease pathology rather than being a result of generalized immunosuppression.
Conceived and designed the experiments: NJS TBN. Performed the experiments: NJS RS SG MLA TBN. Analyzed the data: NJS RS SG MLA TBN. Contributed reagents/materials/analysis tools: NJS RS SG MLA DP TBN. Wrote the paper: NJS RS SG MLA RS MB KP RPB DRM JG TBN.
- 1. Noor A, Knox KS (2007) Immunopathogenesis of sarcoidosis. Clin Dermatol 25: 250–258.
- 2. Zissel G, Prasse A, Muller-Quernheim J (2007) Sarcoidosis–immunopathogenetic concepts. Semin Respir Crit Care Med 28: 3–14.
- 3. Gerke AK, Hunninghake G (2008) The immunology of sarcoidosis. Clin Chest Med 29: 379–390, vii.
- 4. Hedfors E, Holm G, Pettersson D (1974) Lymphocyte subpopulations in sarcoidosis. Clin Exp Immunol 17: 219–226.
- 5. Lower EE, Smith JT, Martelo OJ, Baughman RP (1988) The anemia of sarcoidosis. Sarcoidosis 5: 51–55.
- 6. Selroos O, Koivunen E (1979) Prognostic significance of lymphopenia in sarcoidosis. Acta Med Scand 206: 259–262.
- 7. Kataria YP, LoBuglio AF, Bromberg PA, Hurtubise PE (1976) Sarcoid lymphocytes: B- and T-cell quantitation. Ann N Y Acad Sci 278: 69–79.
- 8. Slade JD, Hepburn B (1983) Prednisone-induced alterations of circulating human lymphocyte subsets. J Lab Clin Med 101: 479–487.
- 9. Baughman RP, Hurtubise PE (1985) Systemic immune response of patients with active pulmonary sarcoidosis. Clin Exp Immunol 61: 535–541.