|
Effect of eliminating intermittent white blood
cells on immunology and cellular factors of
systemic lupus erythematosus
Jin-Jin Jiang, Feng Fang, Lin-Fang Guo and Ruo-Hua Chen
Shanghai, China
Author Affiliations: Changhai Hospital, Second Military Medical University, Shanghai 200433, China (Jiang JJ, Fang F, Gou LF and Chen RH)
Corresponding Author: Jin-Jin Jiang, MD, Changhai Hospital, Second Military Medical University, Shanghai 200433, China (Tel: 86-21-25072117; Fax: 86-21-25070626; Email: jinjinj2000@yahoo.com.cn)
Background: SLE is treated currently by multiple immunosuppression, but side-effects are obvious after long time administration. This study was to observe changes in T, B cells, NK cells and IL12 in patients with systemic lupus erythematosus (SLE) before and after treatment of eliminating intermittent white blood cells and to probe the mechanism of this treatment.
Methods: In 23 patients with SLE, 5 were male and 18 female, with an average age of 15.78±5.40 years. These patients accepted treatment of eliminating intermittent white blood cells. The expressions of CD19+, CD3+, CD4+CD8+, CD4+/CD8+, CD(15+56)+ were tested by flow cytometry before and after the treatment. The amounts of immunoglobulins, IgM, IgG, IgA in periphery blood were measured separately by immunoradiometric analysis before and after the treatment. The level of IL12 was detected by ELISA. Twenty volunteers served as controls.
Results: The expression of CD19+ in the patients increased markedly before the treatment. Statistical significance was noted in the control group and the patient group after the treatment (P<0.01 or P<0.001). The expression of IgM and IgG increased markedly before the treatment. Statistical significance was seen between the control group and the patient group after the treatment (P<0.01 or P<0.001). The expressions of activated CD3+ and CD8+ increased markedly in the patients with SLE before the treatment (P<0.05) (P<0.01 or 0.001) respectively. The expressions of CD3+ and CD4+ decreased markedly (P<0.01 or P<0.05) (P<0.001) respectively. The ratio of CD4+ to CD8+ decreased markedly (P<0.01). The expression of CD3+ after the treatment decreased more remarkably in the patients with SLE than in the control group (P<0.05). The changes in the expression of CD(15+56)+ suggested that the expression of CD(15+56)+ increased markedly before the treatment. Significant statistical difference was observed in the patient group and the control group after the treatment (P<0.05 or P<0.001). The expression of IL12 in the patients with SLE decreased, but it decreased more significantly than in the control group before the treatment (P<0.05 or P<0.01).
Conclusions: Since patients with SLE have the disturbances in T, B cellular immunology and NK cells, IL12, the treatment of eliminating intermittent white blood cells has regulatory effects on T, B cells immunology and NK cells, IL12 in the patients with SLE.
Key words: SLE; immune; NK cell; IL12; eliminating intermittent white blood cells
World J Pediatr 2006;1:53-56
Introduction
Systemic lupus erythematosus (SLE) is one of the autoimmune diseases with unknown causes. The disease is treated currently by multiple immunosuppression, but side-effects are obvious after long time administration. Some immunosuppressants are too expensive to be used in patients with SLE; therefore, researchers are seeking new ways for the treatment of SLE with less side-effects. To increase the efficiency of the treatment, eliminating intermittent white blood cells (WBCs) has been used in patients with SLE at our department since January 2000. The result of this treatment has been significant.[1,2] To probe the mechanism of the treatment, this study focused on the measurements of T, B cell immunity, interleukin 12 (IL12), and NK cells in patients with SLE before and after the treatment.
Methods
Subjects
Twenty-three patients with SLE were admitted to our hospital from January 2000 to December 2003. Among them, 5 were male and 18 female. Their average age was 15.78±5.40 years. The diagnostic criteria were based on Zhu Fu-tang Practical Pediatrics, 6th edition.[3] Twenty volunteers who had normal physical findings as well as normal peripheral blood routine, and liver, renal functions served as controls.
Observation
All 23 patients accepted the treatment of eliminating intermittent white blood cells, using a disposable white blood cell separation device. 200-400 ml blood was taken each time (1-2 times each week; if conditions are stable, 1 time a month), and 4 ml venous blood was taken respectively before and after the treatment of eliminating white blood cells for the assessment of changes in IgG, IgA, IgM, CD3+, CD4+, CD8+, CD4+/CD8+, CD19+, CD(16+56)+ and IL12 in addition to multiple immune indexes and cellular factors. At meantime, 20 samples were taken from the control group consisting of 10 males and 10 females with an average age of 11.42±3.51 years.
Measurement
Lymphocytic subgroups were measured by a FACS calibur flowing cytometer (BD company, USA) with a testing kit of simultestTMIMKPlus (BD company). Immunoglobulins were tested by DADE BehringBNProsel, and IL12 level in plasma was assessed by double antibody ELISA. Immunoglobulins IgG, IgM and IgA were measured by the immunoradiometric assay. Whole blood was stained by the direct double immunofluorescent method and lymphocytic subgroups were measured by a flowing cytometer by adding 20 μl fluorescent labeling monoclonal antibody into 100 µl blood with anti-agglutinant, and reacted for 20 minutes at 4℃. Subsequently, it was centrifuged for 5 minutes at a speed of 1000 r/min while discarding supernatant and washing by PBS solution for two times, and put into a FACS caliber flowing cytometer for regular analysis. With a wavelength of 488 nm, 104 cells were collected from each sample for the measurement of IL12. The sample was centrifuged at a speed of 3000 r/min in a high speed centrifuge. Supernatant was kept, and the sample was placed in a -78℃ freezer for use.
Statistical analysis
All data were expressed by mean ± standard deviation (mean±SD); comparison between the groups was made by Student's t test.
Results
Signs and symptoms of the 23 patients were improved significantly after the treatment. The immune indexes and the level of IL12 also changed.
Changes in B cell immunity
CD19+ before the treatment in the 23 patients was increased more significantly than that after the treatment in the two groups (P<0.01 or P<0.001). The expression of IgM and IgG before the treatment was increased more significantly than that after treatment in the two groups (P<0.01 or P<0.001). The level of IgA increased before the treatment was not significantly different from that after the treatment or from that of the control group. These indexes decreased more significantly than those of the control group after the treatment, but there was no significant difference (Table 1).
Table 1. Results of CD19+ and immunoglobulins IgG, IgM and IgA (mean±SD)
|
Group |
n |
CD19+ (%) |
IgG (g/L) |
IgM (g/L) |
IgA (g/L) |
|
Before treatment |
23 |
23.67±13.85***∆∆ |
20.22±8.01***∆∆ |
1.62±0.72***∆∆ |
1.86±0.73* |
|
After treatment |
23 |
14.61±8.97 |
9.25±3.38 |
1.11±0.62 |
1.60±0.63 |
|
Controls |
20 |
12.05±5.82 |
8.76±2.45 |
1.01±0.43 |
1.21±0.55 |
Compared with control group, *: P<0.05, **: P<0.01, ***: P<0.001; compared with those after treatment, ∆: P<0.05, ∆∆: P<0.01, ∆∆∆: P<0.001.
Changes in T cell immunity
Comparison of the two groups showed the expression of activated CD3+ increased significantly in the patients with SLE before the treatment (P<0.05). The expression of CD8+ increased significantly (P<0.01 or P<0.001), but the expression of CD3+ decreased significantly (P<0.001 or P<0.05). The expression of CD4+ and the ratio of CD4+/CD8+ decreased significantly (P<0.001) (P<0.01) respectively. The expression of CD3+ and the ratio of CD4+/CD8+ in the patients with SLE after the treatment decreased more significantly than in the controls (P<0.05). The expression of activated CD3+, CD4+ and CD8+ was not obviously different from that of the controls (Table 2).
Table 2. Results of CD3+ and activated CD3+ (mean±SD)
|
Group |
n |
CD3+ (%) |
Activated CD3+ (%) |
|
Before treatment |
23 |
63.37±11.66***∆ |
15.08±3.41*∆ |
|
After treatment |
23 |
70.48±7.96* |
8.67±4.25 |
|
Controls |
20 |
78.35±8.56 |
6.08±3.45 |
Compared with controls, *: P<0.05, ***: P<0.001; compared with those after treatment, ∆: P<0.05.
Table 3. Results of CD4+, CD8+, CD4+/CD8+ (mean±SD)
|
Group |
n |
CD4+ (%) |
CD8+ (%) |
CD4+/CD8+ |
|
Before treatment |
23 |
34.61±10.75***∆∆∆ |
42.58±13.21***∆∆ |
0.72±0.42**∆∆ |
|
After treatment |
23 |
47.70±13.31 |
32.39±9.25 |
1.34±0.45* |
|
Controls |
20 |
52.50±8.75 |
31.15±7.25 |
1.40±0.35 |
Compared with controls, *: P<0.05, **: P<0.01, ***: P<0.001; compared with those after treatment, ∆∆: P<0.01, ∆∆∆: P<0.001.
Changes in the expression of CD(16+56)+
The expression of CD(16+56)+ increased significantly before and after the treatment in the controls (P<0.05 or P<0.001) (Table 4).
Table 4. Results of CD(16+56)+ (mean±SD)
|
Group |
n |
CD(16+56)+ (%) |
|
Before treatment |
23 |
7.57±4.10***∆ |
|
After treatment |
23 |
11.65±8.20 |
|
Controls |
20 |
15.76±7.75 |
Compared with controls, ***: P<0.01; compared with those after treatment, ∆: P<0.05.
Changes in IL12
The expression of IL12 decreased more significantly before the treatment in the patients with SLE than in the controls (P<0.05 or P<0.01) (Table 5).
Table 5. Results of IL12 (mean±SD)
|
Group |
n |
IL12 (Pg/ml) |
|
Before elimination of WBC |
28 |
50.21±30.16**∆ |
|
After elimination of WBC |
42 |
65.96±30.10* |
|
Controls |
20 |
169.90±90.02 |
Compared with controls, **: P<0.05; compared with those after treatment, ∆: P<0.05.
Discussion
SLE is characterized by production of autoimmune antibody and abnormal intracellular and extracellular immunological reactions. Patients with SLE have dysfunction of B lymphocytes.[4] As a pancreatic protein in the Tg-SF family, CD19+ is a specific symbol of B cell and a member of the CR2 complex. It can regulate the activation and proliferation of B cell, and participate in the signal transmission of B cell. The abnormality of T cell subgroup may play an important role in inducing the disease.[5,6] The decreased number and dysfunction of T supply cells cause hyperimmune reaction, and the VV- subgroup of CD8+ cell play an inhibitory role. Once the CD8+ VV- subgroup is activated, CD8+ cell as a whole can not express its inhibitory function completely,[7,8] thus leading to the disturbance of the immune system.
NK cells are also important immune regulating cells. The specific symbols of human NK cell surface are CD16 and CD56. NK cells mainly regulate the body immune system by releasing cellular factors which can inhibit the division and proliferation of B cells. They also regulate T cell mediated immunity.[9] In this study, the expression of CD(16+56)+ decreased more significantly in the patients with SLE before the treatment than after the treatment, suggesting the reduced regulation to T, B cells by weakened NK cells. Hence unbalances occurred in T, B, NK cells, resulting in the disturbance of the immune system in patients.
Th1 cellular level and elevated Th2 cellular level were abnormal in the patients with SLE in this group. IL12 is a dimer consisting of two polypeptide chains bonded covalently with one with 3500 aa, and the other with 4000 aa. It is produced after stimulation of antigens by monocytes, macrophages, B cells and other accessory cells.[10] IL12 plays an important role in B cell mediated immune reaction,[11,12] it transforms Th cells to Th1 cells, promotes the proliferation of T cells and NK cells, induces the production of IFN-r, and enhances the division of CTL. The abnormal cellular factors of SLE include mainly reduction of Th1 cellular factor. Patients with SLE often have a reduced level of IL12.[13,14] In this study, the expression of IL12 decreased more significantly before the treatment in the patients with SLE than in the control group.
Previously, eliminating intermittent WBCs was only used in the treatment of hematological diseases and in blood transfusion. Some researchers reported plasma replacement in the treatment of rheumatic diseases,[15] but high medical cost and complications such as disturbance of electrolytes and infections prevented patients with SLE from this treatment. In recent years, stem cell transplantation has been used in the treatment of SLE, but it is expensive and restricted by the source of donors. We have been using the treatment of eliminating intermittent WBC in the treatment of patients with SLE since 2000. The clinical effect of the treatment is satisfactory,[1] and side-effects such as lower proteinemia, disturbance of electrolytes, infections, and hemolysis have been controlled. The clinical signs and symptoms of patients can be improved significantly after the treatment of eliminating intermittent WBCs. Immune index and cellular factor IL12 have been improved simultaneously, elucidating that treatment of eliminating intermittent WBCs regulates T cells, B cells, and IL12 in patients with SLE.
Funding: None.
Ethical approval: Not needed.
Competing interest: None declared.
Contributors: JJJ proposed the study and wrote the draft. FF analysed the data. GLF and CRH provided advices on medical aspects.
References
1 Jiang JJ, Fang F, Guo LF, Shan ZZ, Ou-Yang JH. Therapeutic efficacy of eliminating intermittent white blood cells on rheumatic diseases in children. Chin J Pract Pediatr 2001; 16:735-736.
2 Jiang JJ, Fang F, Guo LF. Cell immune change of eliminating intermittent white blood cells in SLE patients using flow cytometry. J Chin Gen Pract 2003;2:8-9.
3 Zhu FT, Wu RP, Hu YM, Jiang ZF, Mao WH, Wang YX, et al. Practical pediatrics, 6th ed. Beijing: People's Medical Publishing House,1997:647.
4 Scheinecker C, Zwolfer B, Koller M, Manner G, Smolen JS. Alterations of dendritic cells in systemic lupus erythematosus: phenotypic and functional deficiencies. Arthritis Rheum 2001;44:856-865.
5 Robak E, Blonski JZ, Bartkowiak J, Niewiadomska H, Sysa-Jedrzejowska A, Robak T. Circulating TCR gammadelta cells in the patients with systemic lupus erythematosus. Mediators Inflamm 1999;8:305-312.
6 Yu LC, Xiong SD. Molecular immunology: Shanghai Fudan University Publishing House and Shanghai Medical University Publishing House,2001:1127-1211.
7 Zhang DQ, Zhao DF, Zhou GY, Zhang X, Chen SL, Wang Y. VV subgroup of human T cell CD8 manifests reverse inhibition in active patients with SLE. Chin Immunol J 1993; 9:173.
8 Lehner T, Avery J, Jones T. The role of a human antigen specific T8+ cell subset in antigen presentation, helper function and contrasuppression. Clin Exp Immunol 1985;61: 203-213.
9 Eneslatt K, Rantapaa-Dahlqvist S, Uddhammar A, Sundqvist KG. The regulation of Fasl expression distinguishing feature between monocytes and T lymphocytes/NK cells with possible implications for SLE. J Clin Immunol 2001;21: 183-192.
10 Chizzonite R, Truitt T, Podlaski FJ, Wolitzky AG, Quinn PM, Nunes P, et al. IL-12: monoclonal antibodies specific for the 40-kDa subunit block receptor binding and biologic activity on activated human lymphoblasts. J Immunol 1991;147: 1548-1556.
11 Trembleau S, Penna G, Bosi E, Mortara A, Gately MK, Adorini L. Interleukin 12 administration induces T helper type 1 cells and accelerates autoimmune diabetes in NOD mice. J Exp Med 1995;181:817-821.
12 Leonard JP, Waldburger KE, Goldman SJ. Prevention of experimental autoimmune encephalomyelitis by antibodies against interleukin 12. J Exp Med 1995;181:381-386.
13 Min DJ, Cho ML, Cho CS, Min SY, Kim WU, Yang SY, et al. Decreased production of interleukin-12 and interferon-gamma is associated with renal involvement in systemic lupus erythematosus. Scand J Rheumatol 2001;30:159-163.
14 Tyrrell Price J, Lydyard PM, Isenberg DA. The effect of interleukin-10 and of interleukin-12 on the in vitro production of anti-double-stranded DNA antibodies from patients with systemic lupus erythematosus. Clin Exp Immunol 2001;124: 118-125.
15 Suzuki K. The role of immunoadsorption using dextran-sulfate cellulose columns in the treatment of systemic lupus erythematosus. Ther Apher 2000;4:239-243.
Received August 166, 2005; Accepted after revision November 25, 2005
|
