Article Text
Abstract
Objective: To identify clinical and immunological markers of response to treatment with infliximab in ankylosing spondylitis (AS).
Methods: Baseline and sequential cytokine levels (IL1, TNFα, IFNγ, TGFβ and IL10) were examined after 52 weeks of infliximab treatment 5 mg/kg in 22 patients.
Results: At week 52, 18 patients were responders and four non-responders according to ASAS group criteria. Clinical measures of disease activity between the two groups at baseline were similar, apart from a trend towards longer disease duration in non-responders (p = 0.08). Baseline CRP and TNFα levels were higher in responders than non-responders (p<0.01 and p<0.006, respectively). The two groups had similar baseline cytokine levels, apart from TNFα. Baseline CRP levels did not correlate significantly with baseline cytokine levels in responders, but a strong correlation was noted between baseline CRP and IL1, IFNγ, and IL10 in non-responders. Apart from an early rise in TGFβ and a decrease in IL10 in responders after the first infusion, sequential cytokine analysis for the first six months of treatment was not related to clinical disease activity measures.
Conclusion: Although sequential cytokine analysis does not appear to be informative, baseline CRP and TNFα levels are useful markers of clinical response patterns in patients with AS treated with infliximab.
- ankylosing spondylitis
- infliximab
- tumour necrosis factor α
- cytokines
- C reactive protein
- ANOVA, analysis of variance
- AS, ankylosing spondylitis
- ASAS, AS Assessment Study
- BASDAI, Bath AS Disease Activity Index
- BASFI, Bath AS Spondylitis Index
- CRP, C reactive protein
- DMARD, disease modifying antirheumatic drug
- ELISA, enzyme linked immunosorbent assay
- ESR, erythrocyte sedimentation rate
- IFNγ, interferon γ
- IL, interleukin
- NSAID, non-steroidal anti-inflammatory drug
- PBMC, peripheral blood mononuclear cells
- SpA, spondyloarthropathy
- TGFβ, transforming growth factor β
- TNFα, tumour necrosis factor α
- VAS, visual analogue scale
Statistics from Altmetric.com
- ANOVA, analysis of variance
- AS, ankylosing spondylitis
- ASAS, AS Assessment Study
- BASDAI, Bath AS Disease Activity Index
- BASFI, Bath AS Spondylitis Index
- CRP, C reactive protein
- DMARD, disease modifying antirheumatic drug
- ELISA, enzyme linked immunosorbent assay
- ESR, erythrocyte sedimentation rate
- IFNγ, interferon γ
- IL, interleukin
- NSAID, non-steroidal anti-inflammatory drug
- PBMC, peripheral blood mononuclear cells
- SpA, spondyloarthropathy
- TGFβ, transforming growth factor β
- TNFα, tumour necrosis factor α
- VAS, visual analogue scale
Convincing evidence from several short term randomised controlled trials indicates that treatment of ankylosing spondylitis (AS) with biological agents (infliximab and etanercept) is safe and efficacious.1–3 However, a subset of patients fails to respond or does not sustain initial responses. It is thus imperative to define variability in clinical response in order to guide the optimal use of this agent. To date the effect of infliximab on cytokine networks in AS has not been fully defined, although two recent well designed studies have examined the issue.4,5
Neither of these studies, however, aimed at identifying the cytokine profile of patients stratified by response to treatment. Because infliximab is a biological agent that specifically targets tumour necrosis factor (TNF) it seems logical to look for differences in the cytokine profile of patients treated with this agent to identify those patients most likely to respond. In this study we attempt to identify clinical and immunological markers of response to treatment with infliximab in AS. We examined sequential cytokine levels (interleukin (IL) 1, TNFα, interferon γ (IFNγ), transforming growth factor β (TGFβ), and IL10) after 52 weeks of infliximab treatment in 22 patients.
METHODS
Patient ascertainment
Twenty two consecutive patients with AS according to the modified New York criteria6 who had active disease, and for whom non-steroidal anti-inflammatory drug (NSAID) treatment had failed, received infliximab (Remicade; manufactured by Centocor, Malvern, PA and distributed by Schering Plough, Canada Inc) intravenously at baseline, two weeks, six weeks, and every eight weeks thereafter for one year, at a dose of 5 mg/kg. Twenty one of the 22 patients have been described in detail previously.7
The institutional ethics committee reviewed the protocol and all patients signed informed consent.
Laboratory methods
Serial cytokine (IL1, IL10, TGFβ, TNFα, and IFNγ) determinations were measured on peripheral blood mononuclear cells (PBMC) at baseline, weeks 2, 6, 14, and 22. The blood sample was drawn just before the next infusion of infliximab was initiated. PBMC were isolated by Ficoll Hypaque (Pharmacia, Uppsala, Sweden) centrifugation, and resuspended in RPMI. 0.2 ml of the cells was added to a 96 well flat bottomed plate (Costar) at a final concentration of 105 cells per well. The cells were cultured for 48 hours with or without 1 μg/ml phytohaemagglutinin (Gibco BRL). The supernatants were collected and frozen at −60°C.
The respective cytokines were measured by a quantitative sandwich enzyme immunoassay kit (R&D Systems Inc, Minneapolis, MN). All samples were batched and assayed in a single run to minimise interassay variability.
A polyclonal antibody specific for the cytokine to be tested was precoated onto the microplate. Standards and samples were pipetted into the wells and the test cytokine was bound by the immobilised antibody. After washing, the enzyme linked polyclonal antibody against the cytokine was added to the wells. After another wash, a substrate solution was added to the wells and the colorimetric reaction read in an enzyme linked immunosorbent assay (ELISA) reader at 450 nm. Serum levels of cytokines were below the lowest standard within the respective ELISA so supernatants on the stimulated PBMC were the test variables.
C reactive protein (CRP) and erythrocyte sedimentation rate (ESR) were measured by standard laboratory methods.
Primary outcome measures
The following measures were obtained at baseline and each follow up visit: patient global assessment (five point Likert scale: 0 = best, 4 = worst), patient pain (visual analogue scale (VAS): 0 = none, 100 = maximum), Bath AS Functional Index (BASFI) score (0 = none, 100 = worst),8 early morning stiffness (calculated as a mean of the following two scales (a) VAS: 0 = no stiffness, 100 = maximum average early morning stiffness in the preceding week and (b) VAS 100 mm categorical scale of stiffness: 0–120 minutes in 30 minute increments), and physician global assessment (four point Likert scale: 0 = best, 3 = worst).
Response to treatment at week 52 was defined by the AS Assessment Study (ASAS) 20 criteria.9 ASAS response criteria are defined as follows: ⩾20% improvement and an absolute improvement of ⩾10 units in three of four of the following domains: inflammation (early morning stiffness), function (BASFI), patient perception of pain (patient pain VAS), and patient global assessment, with no worsening in the fourth domain. The cohort was divided into two groups according to these criteria at week 52. A cut off point of 50% relative improvement for the ASAS response criteria (that is, ASAS 50 response) was used to stratify the response of the cohort to treatment.
Statistical analysis
The intergroup comparisons of patients’ demographics, disease activity measures, and cytokine levels at baseline were made with independent samples t test. Repeated measures analysis of variance (ANOVA) approach was used to determine whether there were any significant differences between the two groups of patients over the study period.
χ2 Tests (Fisher’s exact test where the assumptions for a χ2 test were not met) were computed to compare change in clinical disease activity (Bath AS Disease Activity Index (BASDAI) or BASFI, ESR, CRP) and candidate cytokines (TGFβ, IFNγ, IL1, IL10, TNFα) in the two groups, after two weeks’ treatment (that is, after the first infusion) and after six weeks’ treatment (that is, after induction of treatment). A p value <0.05 on a two tailed t test was considered significant.
Spearman’s rank correlation coefficient was used to assess the relationship between clinical (BASDAI) or immunological (CRP) measures of disease activity and the candidate cytokines. A correlation coefficient (rs) <0.5 was considered a poor correlation, rs = 0.5–0.7 a moderate correlation, and rs>0.7 was considered a strong correlation. Statistical analysis by intention to treat was performed using SAS (SAS institute Cary, NC version 8.02).
RESULTS
Clinical parameters
At week 52 there were 18 responders and four non-responders by ASAS 20 response criteria. Both responders and non-responders were of similar age (39.7 (8.5) and 40.3 (6.5) years, respectively). Responders had a shorter mean disease duration (9 (7.2) years) than non-responders (16 (5.7) years), which approached statistical significance (p = 0.08). There was no difference in the use of either NSAIDs or disease modifying antirheumatic drugs (DMARDs) between the two groups. Furthermore, there were no discriminating clinical measures of disease activity or function between responders and non-responders at baseline (table 1). There was a difference in inflammatory measures of disease activity (CRP) between the two groups at baseline, with responders having higher CRP levels than non-responders (p<0.01) (fig 1A).
There was a poor correlation between baseline CRP and BASDAI (rs = 0.36) for the whole cohort (of 22 patients), with even lower correlations detected when the cohort was classified into responders and non-responders.
Cytokine analysis
Baseline cytokine levels
Baseline TNFα levels were higher for responders than for non-responders (p<0.006), with the responders having a mean (SD) level of 4797.8 (2793) pg/ml) as compared with (2607 (546) pg/ml) for non-responders (fig 1B). This difference was maintained at the 22 week assessment point (p<0.021). Apart from TNFα, there was no difference between the groups for the remaining baseline cytokine levels.
When response was defined using the ASAS 50 cut off point, there were 12 responders and 10 non-responders at year 1. Although no significant differences in baseline cytokine levels were noted between the groups, responders did have higher baseline TNFα levels (5014 (2805) pg/ml) than non-responders (3662 (2422) pg/ml).
Correlation of clinical and immunological parameters with baseline cytokines
Baseline BASDAI correlated poorly with baseline TNFα (rs = 0.09) for the entire cohort, and for responders (rs = 0.12) and non-responders (rs = 0.10). Similarly, a poor correlation was noted between baseline levels of CRP and the candidate cytokines, for the entire cohort and for responders (figs 2A and B). A strong correlation was noted between baseline CRP and IL1, IL10, and IFNγ levels for non-responders, suggesting that the profile of a non-responder is low baseline CRP, high IL1, high IL10, and low IFNγ levels.
Sequential cytokines
When repeated measures ANOVA testing was used no significant differences were noted between the two groups of patients over the study period at the 0.05 level of significance.
However, a difference by χ2 analysis between responders and non-responders was noted after the first infusion (in the 0–2 week interval) in TGFβ and IL10 levels. During this interval the responders were differentiated from non-responders by higher TGFβ levels and lower IL10 levels. Furthermore, the change in TGFβ and IL10 levels correlated highly with the change in BASDAI but not with CRP. Apart from these observations there was no relationship between response status and change in any of the remaining candidate cytokines over the specified time intervals.
DISCUSSION
In this study we found that patients who respond to infliximab as defined by the ASAS group criteria have higher levels of TNFα and higher CRP levels before treatment than non-responders. The other cytokines studied at baseline—namely, IL1, IL10, IFNγ, and TGFβ, did not differ significantly between responders and non-responders.
The pathogenesis of AS is unexplained and as yet a signature cytokine profile has not been defined in this patient population. TNFα represents a strong candidate as a critical cytokine in the pathogenesis of this disease. Polymorphisms of the TNFα promoter gene have been reported by some groups,10 and local TNFα production has been demonstrated in the biopsies of inflamed sacroiliac joints.11 It is evident from short term trials that therapeutic blockade of TNFα is effective in most patients. But there are clearly patients who do not respond or who fail to sustain their initial response. Our findings suggest that baseline TNFα levels may be an important marker of this effect. On the basis of these findings we suggest that those patients in whom TNFα is lower at baseline the spinal inflammation may not be as TNFα dependent as it is in their counterparts with higher TNFα levels, and that differential response to TNFα blockade is the consequence. This may be explained by the duration of disease in patients where those with longer disease duration have less TNFα dependent spinal inflammation. This hypothesis merits further study with larger numbers of patients as it has important implications for earlier intervention with a TNFα blocker in AS.
Two recent reports have examined changes in cytokines after infliximab treatment in spondyloarthropathy (SpA).4,5 In the first study the cohort was more heterogeneous as the inclusion criteria adopted the European Spondylarthropathy Study Group (ESSG)12 classification of SpA, and cytokines were examined after only short term treatment with infliximab (three infusions). These authors demonstrated an increase in IFNγ after treatment and a decrease in IL10. We did not observe a comparable change in IFNγ, but there were differences in methodology. However, we did notice that there was a difference in IL10, with lower levels in responders than in non-responders after the first infusion. It was also noted in that study that before treatment patients exhibited an impaired Th1 cytokine pattern that was restored after treatment with infliximab. In our study we used each patient as his own control, where the reference point for each treatment interval was each patient’s respective baseline value.
In the second report, 20 patients with AS were selected from a cohort of 70 who participated in a randomised controlled trial.5 Ten of these patients received infliximab for 12 weeks and 10 received placebo for six weeks and were then crossed over to infliximab treatment and evaluated after a further six weeks. The methodology differed from our study in several respects, which obviously makes any comparison between the studies difficult.
Zou et al demonstrated in this study that IFNγ and TNFα secretion from T cells was down regulated significantly by six weeks and this was maintained at 12 weeks after the start of infliximab in the treatment group. In the placebo group no reduction in these cytokines was noted at six weeks, but on cross over to treatment both cytokines decreased significantly at six weeks. Baseline characteristics between groups, including disease activity, were not reported. This may be an important issue as baseline TNFα and IFNγ, seemed to be lower in placebo than in control groups. Possibly, the lack of reduction in TNFα and IFNγ in the patients in the placebo group was due to a floor effect, whereby those patients had significantly lower values than the treatment group. Interestingly, similar to our findings, no significant pattern in sequential cytokine over 12 weeks was detected when evaluation was carried out on peripheral blood monocytes in the patients treated with infliximab.
Neither of the above studies stratified patients according to response to treatment so we do not know whether there were differences in baseline TNFα secretion between responders and non-responders similar to those we found.
In SpA there is no inflammatory marker, such as CRP, that can reliably monitor disease activity.13 Our results are in keeping with this observation, and baseline CRP levels correlated poorly with baseline disease activity. However, the wide variation in CRP levels among the subjects in this cohort might have contributed to the lack of a statistically significant difference. Interestingly, we found that baseline CRP levels were higher in responders than in non-responders. Braun et al made a similar observation on their cohort.1 However, baseline levels of CRP did not correlate with TNFα, which itself was the sole cytokine that distinguished responders from non-responders before treatment. This suggests that there may be an intermediate factor that is related to CRP and TNFα which may predict response also.
In conclusion, this study indicates that measuring CRP and TNFα levels at baseline may be useful in identifying response patterns to infliximab in patients with AS before treatment. On the other hand, sequential cytokine analysis of PBMC does not appear to be informative. Further studies with larger numbers of patients are necessary to perform a multiple logistic regression analysis in order to determine if these variables are true predictors of response to treatment with infliximab.