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This Article Free to Access Abstract Full Text (PDF) All Versions of this Article: ard.2007.080440v1 67/8/1139    most recent Submit a response Alert me when this article is cited Alert me when eLetters are posted Alert me if a correction is posted Services Email this link to a friend Similar articles in this journal Similar articles in PubMed Add article to my folders Download to citation manager Request Permissions Google Scholar Articles by Wijbrandts, C A Articles by Tak, P P PubMed PubMed Citation Articles by Wijbrandts, C A Articles by Tak, P P

The clinical response to infliximab in rheumatoid arthritis is in part dependent on pretreatment tumour necrosis factor expression in the synovium

¹ Division of Clinical Immunology and Rheumatology, Academic Medical Center/University of Amsterdam, Amsterdam, The Netherlands
² Department of Clinical Epidemiology, Biostatistics and Bioinformatics, Academic Medical Center/University of Amsterdam, Amsterdam, The Netherlands
³ Jan van Breemen Institute, Amsterdam, The Netherlands
⁴ Department of Rheumatology, Slotervaart Hospital, Amsterdam, The Netherlands
⁵ VU Medical Center, Amsterdam, The Netherlands

Correspondence to:
Professor P P Tak, Division of Clinical Immunology and Rheumatology, F4-218, Academic Medical Center/University of Amsterdam, Meibergdreef 9 1105 AZ Amsterdam, The Netherlands; P.P.Tak{at}amc.uva.nl

Accepted 18 November 2007

	ABSTRACT

TOP ABSTRACT PATIENTS AND METHODS RESULTS DISCUSSION ACKNOWLEDGMENTS REFERENCES

 
Objective: To determine whether the heterogeneous clinical response to tumour necrosis factor (TNF) blocking therapy in rheumatoid arthritis (RA) can be predicted by TNF expression in the synovium before initiation of treatment.

Methods: Prior to initiation of infliximab treatment, arthroscopic synovial tissue biopsies were obtained from 143 patients with active RA. At week 16, clinical response was evaluated using the 28-joint Disease Activity Score (DAS28). Immunohistochemistry was used to analyse the cell infiltrate as well as the expression of various cytokines, adhesion molecules and growth factors. Stained sections were evaluated by digital image analysis. Student t tests were used to compare responders (decrease in DAS28 1.2) with non-responders (decrease in DAS28 <1.2) and multivariable regression was used to identify the independent predictors of clinical response.

Results: Synovial tissue analysis confirmed our hypothesis that the baseline level of TNF expression is a significant predictor of response to TNF blocking therapy. TNF expression in the intimal lining layer and synovial sublining were significantly higher in responders than in non-responders (p = 0.047 and p = 0.008, respectively). The numbers of macrophages, macrophage subsets and T cells (all able to produce TNF) were also significantly higher in responders than in non-responders. The expression of interleukin (IL)1β, IL6, IL18, IL10, E-selectin, intercellular adhesion molecule (ICAM)-1, vascular cell adhesion molecule (VCAM)-1, vascular endothelial growth factor (VEGF) and basic fibroblast growth factor (bFGF) was not associated with response to anti-TNF treatment.

Conclusion: The effects of TNF blockade are in part dependent on synovial TNF expression and infiltration by TNF producing inflammatory cells. Clinical response cannot be predicted completely, indicating involvement of other as yet unknown mechanisms.

One explanation for the heterogeneous clinical response may be found in the baseline variability in TNF expression among individual patients.^{2 3} Genetic studies have suggested that individuals predisposed to high TNF production could show worse responses to anti-TNF therapy.^{4 5} By contrast, a recent study using an in vitro bioassay suggested that good responsiveness to anti-TNF therapy is associated with significantly higher TNF bioactivity at baseline compared to non-responding patients.⁶ Taken together, it remains to be determined which baseline cytokine profile distinguishes responding from non-responding patients in vivo. Another explanation for the diversity in response may be that inflammatory mediators other than TNF drive different pathogenetic subsets of RA.

We hypothesised that the pretreatment TNF level in the synovium might be related to clinical efficacy, where TNF blocking therapy could be most effective in patients with high pretreatment TNF levels, as previously suggested in a small pilot study.⁷ In a prospective study we obtained arthroscopic synovial tissue samples from 143 patients with RA prior to initiation of infliximab therapy. We examined the cell infiltrate as well as the expression of cytokines, adhesion molecules and growth factors to identify predictors of clinical response.

	PATIENTS AND METHODS

TOP ABSTRACT PATIENTS AND METHODS RESULTS DISCUSSION ACKNOWLEDGMENTS REFERENCES

 
Patients
Consecutive patients with RA according to the American College of Rheumatology (ACR) criteria were enrolled in the study. All failed at least two disease-modifying antirheumatic drugs (DMARDs) including methotrexate (MTX) and had a 28-joint Disease Activity Score (DAS28) of 3.2 when included in the study. Patients were on stable maximal tolerable MTX treatment (5–30 mg/week). Oral corticosteroids (10 mg/day) and non-steroidal anti-inflammatory drug (NSAIDs) were allowed if stable for at least 1 month prior to baseline. Concomitant medication was kept stable throughout the study. Previous use of a TNF blocking agent was an exclusion criterion. The Medical Ethics Committee of the Academic Medical Center, University of Amsterdam approved the protocol. All patients gave written informed consent.

Treatment and evaluation of clinical response
All patients were treated with infliximab according to the label for RA in a dosage of 3 mg/kg intravenously at baseline, week 2, week 6 and subsequently every 8 weeks. The DAS28 was evaluated at baseline and weeks 4, 8, 12 and 16 by specially trained research nurses.

For the analysis the absolute change in DAS28 (DAS28) at week 16 was dichotomised and defined as non-response (DAS28 <1.2) vs response (DAS28 1.2). The dichotomy of the DAS28 (on average comparable with a 20% improvement in DAS28) was chosen because it is applied in daily clinical practice and required for prolongation of reimbursement for TNF blocking therapy by insurance companies in The Netherlands. Response was evaluated at 16 weeks because a significant improvement is expected to occur within 3 to 4 months, after which alternative treatment should be considered.⁸

Arthroscopy and synovial biopsy
Before the first infliximab infusion patients underwent a mini-arthroscopy under local anaesthesia to obtain synovial tissue samples from an actively inflamed knee, ankle, wrist or metacarpophalangeal joint.⁹ Biopsies were taken with 2 mm forceps (Storz, Tuttlingen, Germany) from six or more sites within the joint to minimise sampling error. Biopsies were immediately snap frozen en bloc in Tissue Tek OCT (Miles, Elkhart, Indiana, USA) after collection. Sections of 5 µm were cut in a cryostat and mounted on Star Frost adhesive glass slides (Knittelgläser, Braunschweig, Germany). Slides were stored at –80°C until immunohistochemical staining.

Immunohistochemical analysis
Synovial sections were stained using the following monoclonal antibodies to analyse the infiltrate: anti-CD55 (67:Serotec, Oxford, UK) to detect fibroblast-like synoviocytes (FLS), anti-CD68 (EBM11: DAKO, Glostrup, Denmark) to detect macrophages, anti-CD3 (SK7, Becton Dickinson (BD), California, USA) for T cells, anti-CD22 (CLB-B-ly/1,6B11, The Netherlands) for B cells and anti-CD38 (HB7, BD) for plasma cells. CD163 (Ber-MAC3; DAKO) was stained to detect resident tissue macrophages; infiltrating macrophages were evaluated by detection of myeloid related protein (MRP)8 (8-5c2, BMA Biomedicals, Augst, Switzerland) and MRP14 (S36.48, BMA Biomedicals). For the detection of cytokines, adhesion molecules and growth factors we used anti-human TNF (52B83; Monosan, Brussels, Belgium), anti-interleukin (IL)6 (Nephrology Department, Leiden University Medical Center, Leiden, The Netherlands), anti-IL10 (23738.111, R&D, Abingdon, UK), anti-IL18 (2d3b6, MD Biosciences, Minnesota, USA), anti-IL1β (2D8, ImmunoKontact, Oxford, UK), anti-intercellular adhesion molecule (ICAM)-1 (MEM111, Sanbio, Erembodegem, Belgium), anti-vascular cell adhesion molecule (VCAM) (1G11B1, Sanbio), anti-E-selectin (BBIG-E4, R&D), anti- vascular endothelial growth factor (VEGF) (N.010313 C-1, Santa Cruz, California, USA) and anti-basic fibroblast growth factor (bFGF) (F14220, BD). Staining of cellular markers was performed using a three-step immunoperoxidase method.² For staining of cytokines, adhesion molecules and growth factors, biotinylated tyramine was used as amplification. For control sections the primary antibody was omitted or irrelevant immunoglobulins were applied.

Digital image analysis
All sections were analysed at random by trained analysts blinded for clinical outcome. Images were acquired and analysed by computer-assisted image analysis using a Syndia algorithm on a Qwin-based analysis system (Leica, Cambridge, UK).¹⁰ A total of 18 high-power fields per marker were analysed. Cellular markers were expressed as positive cells/mm² (counts/mm²). Staining of cytokines, adhesion molecules and growth factors was expressed as integrated optical density/mm² (IOD/mm²). CD68+ macrophages and TNF expression were analysed separately in the intimal lining layer and the sublining.

Statistical analysis
Independent Student t tests or Mann–Whitney U tests were used to detect significant differences in baseline parameters between responders and non-responders. The ² test was employed to compare the percentage of erosive, IgM-rheumatoid factor (RF) and anti-cyclic citrullinated peptide (CCP) positive patients in the responder and non-responder groups. Variables with a p value <0.1 in the univariable analysis were selected as possible predictors in a stepwise backward multivariable logistic regression model. Several exchangeable prediction sets were constructed based on the correlation structure among the potential predictors with strongly correlating predictors in different sets. The model with the highest explained variance according to Nagelkerke is reported. Correlations were assessed with the Pearson product-moment or Spearman rank-order correlation coefficients, whichever was appropriate. SPSS V.11.1.4 (Chicago, Illinois, USA) was used. Because the primary objective of this study was to find a pathogenetic mechanism in synovial tissue relating to clinical response, a per-protocol analysis was performed.

	RESULTS

TOP ABSTRACT PATIENTS AND METHODS RESULTS DISCUSSION ACKNOWLEDGMENTS REFERENCES

 
Enrolment, discontinuation and exclusion
A total of 143 patients were enrolled. The population was predominantly female (74%), RF positive (71%) with a mean (SD) age of 55 (13) years and mean disease duration of 125 (108) months. Erosions were present in 110 (77%) patients. The mean DAS28 score was 5.9 (1.0) at baseline and the mean MTX dose was 18.2 (8.5) mg/week. In three patients, a flare of arthritis at week 6 (n = 1) and week 12 (n = 2) was the reason for discontinuation. These patients were analysed as non-responders. Patients (n = 18) who violated the protocol or discontinued infliximab therapy (for reasons other than non-response) were excluded.

Synovial tissue exclusion
Following strict quality control, 23 synovial biopsies were excluded by a blinded assessor for absence of an intimal lining layer. After excluding 18 patients from the response analysis and 23 synovial biopsies from the tissue analysis a total of 103 completely evaluable patients remained for the analysis of synovial tissue in combination with clinical response.

Baseline patient characteristics
The remaining group of 103 patients who were analysed for response in combination with synovial tissue consisted of 71 females and 32 males, of whom 75% were rheumatoid factor positive. The mean (SD) age was 55 (13) years and the mean disease duration was 125 (110) months. Erosions were present in 79 (77%) patients. The mean DAS28 score was 5.9 (1.1) at baseline and the mean MTX dose was 18.8 (8.5) mg/week. Corticosteroids were used by 28 (27%) patients with a mean dose of 8.0 (2.9) mg/day. On average, patients had failed treatment with 2.2 DMARDs before inclusion in the study. No notable changes occurred in the baseline characteristics of the analysed 103 patients compared to the baseline characteristics of all 143 enrolled patients (see table 1).

All baseline patient characteristics were also tested for differences between responders and non-responders. The DAS28 at baseline was nearly significant and was included in the prediction model (p = 0.07). The same holds for anti-CCP positivity (p = 0.08). Finally, there were significantly more rheumatoid factor positive patients in the responder compared to the non-responder group (p = 0.020), (see table 1).

Baseline synovial TNF expression and the number of major TNF producing cells are associated with clinical response (DAS28 1.2) after 16 weeks of TNF blocking therapy
Scatter diagrams of the synovial predictors in individual patients in both response groups are presented in fig 1. TNF expression levels were higher in the synovial sublining of responders compared to non-responders (p = 0.008) (fig 1A). Similarly, TNF expression in the intimal lining layer was higher in responders compared to non-responders (p = 0.047). Table 2 shows the associations of synovial markers and response.

View larger version (29K): [in this window] [in a new window] [PowerPoint for Teaching]   Figure 1 A. The median synovial sublining tumour necrosis factor (TNF) expression was higher in responders compared to non-responders (p = 0.008). B. The median number of CD3+ T cells in responders vs non-responders (p = 0.001). (C) The mean number of CD68+ sublining macrophages was also higher in responders 576 (428), than in non-responders 387 (338) (p = 0.029). (D) CD163+ macrophages in responders vs non-responders (p = 0.017).

Baseline TNF is the only significant synovial predictor of response
The relationship between TNF expression and clinical response was confirmed by stepwise backward multivariable logistic regression analysis. Due to multicolinearity among predictors, 10 exchangeable bivariate prediction sets were constructed consisting of (1) TNF expression in either the intimal lining layer or synovial sublining with (2) one out of five cellular markers. This revealed that TNF expression in the synovial sublining was the only independent, early determinant of therapy response (p = 0.011), explaining just about 10% of the variance in response to therapy (R² = 0.099, according to Nagelkerke, odds ratio (OR) = 1.013). Likewise, TNF expression in the intimal lining layer rather than synovial sublining explained 9% of the variance in response to therapy (p = 0.020), (R² = 0.089, OR = 1.017). Thus, after adjustment for TNF in a bivariate logistic regression model including either the numbers of CD68+ sublining macrophages, CD163+, MPR8+, MRP14+ macrophages, or CD3+ T cells, these cellular markers were no longer significantly associated with response. The removal of these cellular markers from the model is consistent with the notion that these cells are the main producers of TNF.

Contribution of disease activity at baseline to the prediction of response
To assess the value of a combined prediction model consisting of clinical and synovial data we added the relevant clinical variables (DAS28 score, the presence of IgM-RF or anti-CCP antibodies) to the 10 bivariate synovial models. With stepwise backward multivariate logistic regression this resulted in a significant prediction model with TNF expression in the synovial sublining (p = 0.008, OR = 1.014) and the DAS28 (p = 0.031, OR = 1.611) with an increased explained variance of 17% (R² = 0.172). A similar analysis except with TNF expression in the intimal lining layer (p = 0.023, OR = 1.017) resulted in a significant model including the DAS28 (p = 0.044, OR = 1.588) and the presence of anti-CCP antibodies (p = 0.046, OR = 3.038) (R² = 0.182).

Baseline IL1β, IL6, IL18 and IL10 expression is not associated with response to TNF blocking therapy
In addition to TNF we studied the expression of other cytokines such as IL18, which is believed to operate mainly upstream of TNF, while IL1β and IL6 appear to act mainly downstream of TNF. Despite the known interplay of these cytokines with TNF we found no relationship between synovial expression levels of either of these cytokines and clinical response. We did find, however, a significant correlation between the level of IL1β expression and TNF expression (r = 0.306, p = 0.014). The expression level of IL10 was not different between response groups (see table 2).

Baseline expression of adhesion molecules and angiogenic factors is not associated with response to TNF blocking therapy
In accordance with their function in leukocyte recruitment a significant correlation was found between the number of sublining macrophages on the one hand and the expression of the vascular adhesion molecules E-selectin (Spearman rho correlation coefficient 0.275–0.536, p<0.01) on the other. However, the level at which the adhesion molecules were expressed in the synovium at baseline did not differ between responders and non-responders. Furthermore, VEGF is known to mediate angiogenesis and is regulated by pro-inflammatory cytokines such as TNF. However, no association was found between VEGF expression and response (table 2). Similarly, no difference was found in the expression of bFGF.

	DISCUSSION

TOP ABSTRACT PATIENTS AND METHODS RESULTS DISCUSSION ACKNOWLEDGMENTS REFERENCES

 
The primary objective of this study was to investigate whether immunohistological assessment of the cell infiltrate and cytokine expression in the synovium prior to initiation of TNF blocking therapy could predict clinical response in patients with RA. We could confirm our hypothesis that the level of synovial TNF expression is a significant early predictor of the response. This was shown by increased TNF expression levels in the intimal lining layer and synovial sublining of responding compared to non-responding patients. In line with these findings, there was increased infiltration by macrophages, including CD163+ resident tissue macrophages and MRP8+ and MRP14+ infiltrating macrophages, as well as T cells in responders vs non-responders. It is important to note that these cells are the main source of TNF in the synovium of patients with RA.¹¹

Consistent with the clinical experience that the response to TNF blockade is not a dichotomous phenomenon,¹² there was no distinct threshold value in TNF expression in the synovium of patients with RA. Multivariate logistic regression analysis of synovial markers showed that TNF expression in the sublining could explain about 10% of the variance in response to therapy. After adjusting for disease activity at baseline this further increased to 17%. Hence, the predictive value of synovial TNF expression is statistically significant, but overall limited. This clearly indicates that variables other than synovial TNF expression are involved as well. The results presented here show for the first time that the expression of IL1β, IL6, IL18, IL10, E-selectin, ICAM-1, VCAM-1, VEGF and bFGF is not associated with clinical response to anti-TNF treatment. Thus, the features of synovial inflammation at baseline in responders to anti-TNF therapy compared to non-responders do not merely represent a greater amount of inflammation, but the results presented here underscore the importance of specific inflammatory pathways. Future work should expand the search for other biomarkers and molecular networks to better understand the variable response to anti-TNF therapy.

The search for predictors of response is important in the context of personalised medicine, which may be an effective approach to increase the percentage of patients exhibiting a robust response to a given treatment. Previous work has clearly suggested that RA consists of different pathogenetic subsets, leading to common signs and symptoms associated with what we at present define clinically as RA.^{2 3 13} Thus, it is conceivable that, for instance, TNF expression is more important in some patients than in others, and that TNF blockade could be more effective in the former. Although we are as yet not able to predict the response sufficiently to select patients who are likely to have a beneficial response to a specific treatment before initiation of therapy and to guide treatment decisions, the results of the present study do provide proof of principle that this might be achieved by further optimisation of the biomarkers or perhaps combinations with other clinical and biological variables that need to be identified. The relevance of this approach is underscored by the expanding array of biological therapies and their costs.¹⁴

There is no evidence that simple measurement of plasma TNF levels can be used to predict clinical response to TNF blockade. As it appears logical that patients producing high levels of TNF at the site of inflammation are more likely to benefit from TNF blockade than those with lower TNF levels, we focused on the synovium as the primary target of RA. The association between pretreatment TNF expression in the synovium and clinical response to 3 mg/kg of infliximab described here in 103 patients with RA confirms and extends a trend observed in a pilot study in patients with RA where 4 out of 8 patients who met the ACR50 response criteria at 2 weeks after initiation of infliximab (10 mg/kg) therapy were those with the highest levels of TNF expression in the synovium, as shown by immunohistochemistry.⁷ Of interest, the findings are also in accordance with a recent study suggesting that clinical response at 52 weeks is associated with significantly higher circulating TNF bioactivity (measured by an in vitro bioassay) at baseline in responding compared to non-responding patients.⁶ Together, these studies support the notion that the initial clinical response to TNF blockade is related to pretreatment levels of TNF production. In patients who initially respond, but loose response over time, other mechanisms such as formation of antibodies against the drug may be operative.¹⁵

In conclusion, the results presented here show proof of principle that the heterogeneous response to TNF blockade is associated with TNF expression in the inflamed synovium. Future work should expand the search for other biomarkers and molecular networks as well as combinations with clinical variables. Thus, the prediction of how a patient will respond might come in reach of the treating doctor.

	ACKNOWLEDGMENTS

TOP ABSTRACT PATIENTS AND METHODS RESULTS DISCUSSION ACKNOWLEDGMENTS REFERENCES

 
The authors wish to thank Professor A H Zwinderman, head of the department of Department of Clinical Epidemiology, Biostatistics and Bioinformatics at the Academic Medical Center/University of Amsterdam, for reviewing the statistical analysis. We also wish to thank Desiree Pots for assisting with the immunohistochemical staining, and research nurses Nitolanda van Rijn and Natasja Cassin for performing clinical assessments.

	FOOTNOTES

 
Funding: This study was funded by a Health Care Efficiency Research Programme grant from The Netherlands Organization for Health Research and Development (ZonMw) in assignment of The Netherlands Organization for Scientific Research (NWO) (grant number 945-02-029), the Dutch Arthritis Association and the European Community’s FP6 funding (Autocure).

Competing interests: PPT has served as a consultant for Abbott, Amgen, Centocor and Wyeth.

Ethics approval: The Medical Ethics Committee of the Academic Medical Center, University of Amsterdam approved the protocol. All patients gave written informed consent.

This publication reflects only the authors’ views. The European Community is not liable for any use that may be made of the information herein.

Published Online First 29 November 2007

	REFERENCES

TOP ABSTRACT PATIENTS AND METHODS RESULTS DISCUSSION ACKNOWLEDGMENTS REFERENCES

 

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This Article Free to Access Abstract Full Text (PDF) All Versions of this Article: ard.2007.080440v1 67/8/1139    most recent Submit a response Alert me when this article is cited Alert me when eLetters are posted Alert me if a correction is posted Services Email this link to a friend Similar articles in this journal Similar articles in PubMed Add article to my folders Download to citation manager Request Permissions Google Scholar Articles by Wijbrandts, C A Articles by Tak, P P PubMed PubMed Citation Articles by Wijbrandts, C A Articles by Tak, P P