First Department of Medicine, University of Mainz, Mainz and 1 Dialysis Practice, Ingelheim, Germany
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Abstract |
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Methods. Thirteen patients with ESRD on intermittent haemodialysis treatment, six patients with chronic renal failure not yet on dialysis, and 15 age- and sex-matched healthy controls were examined. Monocytes, purified from peripheral blood mononuclear cells (PBMC) by immunomagnetic bead separation, were incubated for 18 h in the presence of MSU crystals, Escherichia coli lipopolysaccharide (LPS) or medium alone. The supernatants were studied for the presence of interleukin (IL)-1ß, IL-6 and tumour necrosis factor- (TNF-
) using cytokine-specific enzyme-linked immunosorbent assays.
Results. Monocytes from patients with ESRD produced significantly lower amounts of IL-1ß, IL-6 and TNF- after stimulation with MSU crystals or LPS than did monocytes from healthy subjects. Cytokine production was not significantly different between ESRD patients on haemodialysis and chronic renal failure patients not yet on dialysis. Artificial MSU crystals were stronger stimuli than tophus-derived natural MSU crystals.
Conclusion. We demonstrate that monocyte-associated immunosuppression in ESRD leads to reduced secretion of proinflammatory cytokines in response to stimuli such as MSU crystals. This may be one of the factors preventing many ESRD patients from the manifestation of acute gout despite often severe hyperuricaemia.
Keywords: cytokines; end-stage renal disease; gout; monocytes; monosodium urate crystals
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Introduction |
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It is known that in gouty arthritis, monosodium urate (MSU) crystals interact with monocytes, neutrophils and endothelial cells to produce inflammatory reactions associated with acute synovitis [10]. Among the factors that regulate the grade of inflammation in joints that contain MSU crystals, coating of the crystals by different proteins may be one important modulating mechanism [11]. Secondly, MSU crystals and other inorganic crystals have been shown to induce the formation of specific antibodies which in turn can catalyse the more rapid formation of new crystals [12,13]. Thirdly, a balance between various cytokines and other molecules that exert pro- and anti-inflammatory effects has been incriminated in the modulation of MSU crystal-associated synovitic inflammation. Neutrophils and endothelial cells may be a source of oxygen radicals in crystal-induced inflammation, since these cells phagocytose MSU crystals and produce superoxide anion [14]. Monocytes exposed to MSU crystals secrete interleukin-1 (IL-1), tumour necrosis factor- (TNF-
) and interleukin-6 (IL-6) [15,16] which cause both local inflammation and systemic manifestations including fever and elevated C-reactive protein [17]. In contrast, regulatory synovial cytokines such as transforming growth factor-ß1 (TGF-ß1) may down-regulate actue and chronic inflammation [18].
Here we analyse crystalcell interactions in patients with ESRD compared with age-matched healthy controls and test the hypothesis that suppression of proinflammatory cytokine responses due to an uraemia-associated monocyte immune deficiency may be one explanation for the relatively low incidence of gout in patients with long-standing renal insufficiency.
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Subjects and methods |
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MSU crystals
Artificial MSU crystals were prepared under pyrogen-free conditions from a supersaturated solution of sodium urate as described [19]. Natural MSU crystals were obtained from a tophus surgically removed from a patient suffering from gout, purified as described and washed in phosphate-buffered saline (PBS) [20].
Isolation of peripheral blood monocytes
Mononuclear cells (MNC) were isolated from heparinized blood by standard Ficoll-Hypaque density centrifugation (Histopaque-1077, Sigma, Deisenhofen, Germany). In HD patients, blood was drawn directly before HD started in order to avoid monocyte activation by the procedure of HD. In the first series of experiments, various methods for the purification of human monocytes from MNC were evaluated: the E-rosetting technique to enrich monocytes and B-lymphocytes and remove T cells, Percoll density gradient centrifugation, counterflow centrifugal elutriation and immunomagnetic separation (IMS). The aim of these evaluation experiments was to achieve a pure population of monocytes with minimum pre-activation due to plastic adherence or other in vitro manipulations. The monocytes should also be stimulated optimally by mitogens and by MSU crystals.
The E-rosetting technique to enrich B cells and monocytes
MNC (5x107) were resuspended with 2 ml of a prepared solution of 300 µl of sheep erythrocytes incubated with 100 µl of Test-Neuraminidase (Centeon, King of Prussia, PA, USA) in 4.6 ml of RPMI-1640 (Seromed, Berlin, Germany) for 30 min at 37°C, layered on Ficoll 1.090 (Biochrom, Berlin, Germany) and centrifugated for 30 min at 2800 r.p.m. [21]. The interface layer containing B cells and monocytes was collected and washed with PBS/3% fetal calf serum (FCS).
Percoll density gradient centrifugation
MNC (5x107) were suspended in 2 ml of a 100% Percoll solution (Percoll, Sigma, Deisenhofen, Germany) in a 15 ml centrifuge tube and overlayered by Percoll gradients containing 3 ml layers of 60, 50 and 35% of Percoll in PBS. After centrifugation for 20 min at 3000 r.p.m. and 4°C, the monocytes were collected from the interface between the 60 and the 50% layer and were washed with PBS/3% FCS.
Counterflow centrifugal elutriation
A J2-MC Elutriator system (Beckmann, Munich, Germany) was treated with PBS/1% bovine serum albumin (BSA) to block unspecific binding sites and then washed with elutriation buffer (PBS). The elutriation of monocytes was performed according to a method described by Fidgor et al. [22] and to the manufacturer's instructions at 1600 r.p.m. and 16°C. At an initial flow of 20 ml/min, remaining red blood cells and detritus were removed from the elutriation chamber. Thereafter, 1000 ml of a cell mixture of lymphocytes and a few monocytes was collected at a flow of 29 ml/min. The monocytes were finally collected at a flow of 50 ml/min into 50 ml tubes and kept on ice until they were centrifuged for 10 min at 1200 r.p.m. and 4°C and resuspended in Dulbecco's modified Eagle's medium (DMEM; Gibco, Eggenstein, Germany) containing 10% heat-inactivated human AB serum.
Immunomagnetic separation of monocytes
IMS was performed using Dynabeads according to the manufacturer's instructions (Deutsche Dynal, Hamburg, Germany). Briefly, Dynabeads M-450 were washed twice in PBS/3% FCS using a Dynal MPC-1 magnetic separation device. Peripheral blood MNC (PBHC) prepared by the E-rosetting technique were suspended in PBS/3% FCS at 2x107 cells/ml in a 15 ml conical tube, and the pre-washed Dynabeads M-450 were added together with anti-CD2 and anti-CD19 monoclonal antibodies (Immunotech, Hamburg, Germany). After incubation at 4°C for 30 min with gentle tilting and rotation, the tubes were placed in a Dynal MPC for 2 min to remove magnetically the CD2+ and CD19+ cells coated with beads. The unbound, negatively selected cells were transferred to a fresh tube, and a second magnetic separation procedure was performed. The resulting cells were counted, and resuspended in DMEM (Gibco) containing 10% heat-inactivated human AB serum.
Monocyte stimulation by MSU crystals and lipopolysaccharide
Freshly isolated blood monocytes (0.5x106 cells per well) were cultured with the various stimuli (artificial and natural MSU crystals at different concentrations, purified lipopolysaccharide (LPS) from Escherichia coli, (Sigma, Deisenhofen, Germany) or culture medium alone) in 48-well flat bottom plates (Greiner, Nürtingen, Germany) for 18 h. An incubation time of 18 h was found to induce peek levels of cytokine secretion by the monocytes. The supernatants were collected, centrifuged to remove crystals and cell debris, and stored at -80°C until they were tested for the presence of cytokines.
ELISAs for IL-1ß, IL-6 and TNF-
Maxi-Sorb 96-well plates (Nunc, Roskilde, Denmark) were coated with 2 µg/ml of anti-IL-1ß (Immunotech, Hamburg, Germany), anti-IL-6 (Virotech, Rüsselsheim, Germany) or anti-TNF- (Biozol, Munich, Germany) monoclonal antibodies, respectively. After washing, excess sites were blocked with 100 µl of 5% BSA (Serva, Heidelberg, Germany) in PBS. After subsequent washing with PBS/0.05% Tween, the reaction mixtures (100 µl of culture supernatants) were pipetted into triplicate wells; standards were always included in the same trays. The plates were incubated overnight and washed four times, followed by incubation with 100 µl of biotinylated rabbit anti-human IgG (2 µg/ml) (Serva) and subsequently with 100 µl of avidin-conjugated peroxidase (1 µg/ml) (Dako, Hamburg, Germany). Finally, substrate ABTS (Serva) was added. Colour development was measured by determining the optical density at 405 nm with an automated microplate reader.
Statistical analysis
The data were analysed using the KruskalWallis test and the Wilcoxon test according to the advice of the Institute of Medical Statistics and Documentation, University of Mainz. The significance level was P<0.01.
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Results |
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Cytokine release of monocytes depending on the purification method used
The different separation methods were also compared in order to evaluate the extent of monocyte pre-activation during these procedures and the optimal activation after mitogen or MSU crystal stimulation by measuring the cytokine release. Monocyte isolation by Percoll led to higher production of IL-1ß, IL-6 and TNF-, (data shown for TNF-
, see Figure 1
) in unstimulated cells (medium) than counterflow centrifugal elutriation, E-rosetting or IMS. In contrast, Percoll isolation of monocytes induced the highest spontaneous levels of the three cytokines (medium control). Therefore, for further experiments, the IMS method was chosen, since it showed high monocyte purity after isolation (see Table 1
) and led to very low spontaneous but high LPS- or MSU crystal-inducible cytokine secretion, thus resulting in an optimal stimulation index.
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Monocyte IL-1ß, IL-6 and TNF- secretion induced by MSU crystals and LPS
Monocytes separated by immunomagnetic beads spontaneously released only very low amounts of cytokines. When the cells were stimulated with LPS or various amounts of artificial and natural MSU crystals, the cytokine secretion was significantly increased. In these experiments, stimulation with artificial MSU crystals was more effective than stimulation with microcrystals that had been prepared from a tophus (natural MSU crystals) (Figure 2).
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Discussion |
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The results found here in the group of healthy subjects are in concordance with previous work on the stimulatory effect of MSU crystals on IL-1 and IL-6 release from monocytes [17]. These studies demonstrated that within hours after incubation with MSU crystals, monocytes produced proinflammatory cytokines and expressed cyclooxygenase-2 [23]. In addition, MSU crystals could activate endothelial cells [24]. The resultant release of inflammatory mediators from the endothelium and from monocytes is believed to be important in specific aspects of the pathogenesis of gout including acute local synovitic inflammation and systemic acute phase responses.
Concerning patients with ESRD, the working hypothesis of our present work has been that suppression of the proinflammatory cytokine response due to an uraemia associated monocyte immune deficiency might be one explanation for the relatively low incidence of gout in long-standing renal insufficiency. Several previous studies have suggested that ESRD induces a clinical state of immune deficiency, including an increased incidence of bacterial and fungal infections, an impaired efficacy of vaccinations such as hepatitis B [25] and clinical and serological remissions of systemic lupus erythematosus (SLE) as azotaemia develops [26]. In vitro, impaired T cell-mediated immune responses in ESRD are based mainly on reduced T cell-activating capabilities of monocytes [27], an involvement of the B7/CD28 pathway [28] as well as enhanced monocyte apoptosis [29].
Our findings of significantly reduced cytokine production by MSU crystal-stimulated monocytes from patients with ESRD provide direct support for the hypothesis that the ability of monocytes to secrete proinflammatory cytokines is critical in the clinical state of ESRD-induced immunodeficiency. Moreover, not HD but azotaemia itself seems to be responsible for the defect of monocytes in ESRD, as demonstrated by the fact that there were no significant differences in cytokine production in patients with ESRD on intermittent HD and patients with chronic renal failure not yet on dialysis. This correlates with the general lack of prominent systemic acute phase responses in many patients with long-standing renal insufficiency. Our findings may in part explain the observation that despite hyperuricaemia in chronic azotaemia and despite the formation of MSU crystals, acute inflammatory gouty arthritis is extremely rare in ESRD and the clinical course is ameliorated in those patients who have had a history of gout in the stage of early renal insufficiency [7].
Measurement of cytokines in patients with ESRD has been performed by several groups and, unfortunately, the results are contradictory. Pereira et al. [30] compared different studies on cytokine secretion in patients on HD and tried to find out the reasons for the inconsistent findings. They made clear that the results strongly depended on the method of cell separation used, the purity and pre-activation of the cell population as well as the method of cytokine measurement. These aspects were taken into consideration in our present study. We found that monocyte pre-activation due to the separation procedures was crucial for the amount of proinflammatory cytokines detected by ELISA pre- and post-stimulation with LPS or MSU crystals. Therefore, we would suggest choosing for further studies in this field the IMS method (negative isolation by antigenantibody reactions) to separate monocytes from an MNC fraction.
Interestingly, natural MSU crystals were biologically much less active than synthetic counterparts (artificial MSU crystals), which was in contrast to the findings of Stankovic et al. [20]. It should be noted, however, that these human crystals were obtained from tophi in the skin where they are known to evoke little, if any, inflammation aside from phagocytosis by macrophages.
In summary, the findings presented here may represent one aspect of how proinflammatory monocyte reactions in response to MSU crystals and the resulting acute gouty arthritis might be prevented in patients with ESRD. Differences between ESRD patients and healthy controls may also involve differences in MSU-induced complement activation, neutrophil and endothelial stimulation or T cell mitogenesis. The effects of MSU on neutrophil activation in ESRD patients are now under investigation in our laboratory.
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Notes |
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References |
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