Background
In multiple sclerosis (MS) patients, IFNβ-1a reduces clinical and imaging signs of disease activity, ultimately delaying the progression of physical disability [
1,
2].
However, a relatively long-term follow-up is necessary for changes in physical disability scores to become evident. Although magnetic resonance imaging (MRI) represents a gold standard for MS diagnosis and can provide fast information regarding the stage of the disease and its changes over time, is still an expensive and time consuming test. Inarguably, a biological marker of drug response would provide a low-cost and easy method of assessing treatment efficacy. To date, no biomarkers that parallel clinical and MRI measurements of response to treatment have been identified. Several lines of evidence suggest that neopterin and tryptophan (trp) degradation catabolites (such as kynurenine [kyn]) could be considered indirect indicators of IFNβ's action [
3‐
5].
Binding of IFNβ to its cell-surface receptor stimulates several immunological processes, including neopterin [D-
erythro-6-(1',2',3'-trihydroxypropyl)-pterin] production [
6] and trp degradation [
7,
8].
In vitro evidence demonstrated that both IFNβ and IFNγ induce neopterin production [
9] and activate the enzyme indoleamine (2,3)-dioxygenase (IDO). Such enzyme catalyzes trp degradation to kyn (among other downstream catabolites) in several cell types [
10,
11]. The kyn/trp ratio provides an estimate of IDO activity and correlates with markers of IFNγ immune activation, like neopterin [
8,
12].
While neopterin has numerous biochemical and physiological functions in host defense, trp degradation induced by IDO limits trp supply for proliferating cells, thus determining their growth arrest [
8,
13,
14]. Hence, neopterin production and trp degradation could be considered as indicators of the antiviral and immunomodulatory activities of type-I IFNs.
In vivo studies in MS patients have confirmed that IFNβ-1a induces neopterin production [
15‐
17] and IDO activation [
18]. However, it remains unknown if any of those markers correlates with IFNβ-1a dose and/or clinical outcome.
In this prospective study 101 patients with relapsing remitting MS (RRMS) were treated with one of two doses of IFNβ-1a for 24 months. Repeated evaluations of neopterin and kyn/trp ratio, as well as of physical disability, were performed in order to assess the correlation between biological and clinical effects of IFNβ-1a in these patients. The correlation between the markers of IFNβ biological activity and the presence of neutralizing antibodies (Nabs) [
19,
20] was also evaluated.
Methods
Study design
This open-label randomized study was conducted in seven Italian academic MS clinical centers (University Hospitals of Chieti, Firenze, Isernia, L'Aquila, Messina, Roma, and Trieste), in collaboration with the University of Innsbruck in Austria and the National Institute of Biological Standards and Control in London, UK.
The study consisted of a 12-months screening/enrollment phase, followed by a 24-months follow-up treatment phase (TP), during which IFN-naïve RRMS patients received IFNβ-1a, either 22 mcg (low-dose, LD) or 44 mcg (high-dose, HD) subcutaneously (sc) three times weekly. Given the spontaneous, non-interventional design of the study, in order not to modify common clinical practice, but to warrant at the same time an evenly distributed study population, the dose of IFNβ-1a considered optimal by the treating physician was first started. Patients were then randomized, through a centralized procedure, to be included or not included in the study, maintaining the dosage selected by the treating physician, i.e. a patient was excluded from the study if the selected dosage did not agree with randomization. Care was taken as to reach a balanced sample of LD- and HD-patients (i.e., ~40 to 60% in each group) at each site.
All patients underwent a full clinical examination rating their physical disability, by the Expanded Disability Status Scale, or EDSS score [
21], before treatment (referred as baseline thereafter). After the baseline visit, clinical assessments were repeated every 6 months. An additional clinical examination was performed when a clinical relapse occurred, defined as the occurrence of a new symptom or worsening of a pre-existing symptom, lasting at least 48 hours in the absence of fever [
22]. Relapses were treated with intravenous methylprednisolone (MP), 1 g/d for 5 days.
At baseline and every 3 months thereafter, blood samples were collected between 8:00am and 1:00 pm, in fasting conditions. The post-dose time was 60-65 hours after the last IFNβ-1a injection. Such interval was chosen based on previous observations that neopterin values remained significantly elevated 48-72 hours after administration of IFNβ-1a both in healthy subjects [
23] and in patients with MS [
16]. The chosen time interval aimed at both maximizing the timing of sample collection consistency and, at the same time, accommodating patients' availability. As cytokine levels may vary throughout the day, all samples were collected at the same time of the day for each patient.
Blood samples were not collected if clinically evident inflammation/infection was present. In those cases samples were collected 2 weeks after symptom resolution.
Inclusion and exclusion criteria
Patients with RRMS, according to the Poser's criteria [
24], were recruited. Other inclusion criteria were age 18-50 years, body weight within 15% of normal (minimum weight: 50 kg), disease duration ≤ 10 years, at least two relapses in the preceding 2 years, EDSS score of 1.0-5.5. Exclusion criteria were clinical relapse at the time of enrollment; corticosteroid treatment within 1 month, immunomodulatory or immunosuppressive therapy within 6 months prior to study entry, pregnancy, major psychiatric disturbances, and other neurological, neoplastic, autoimmune or major infectious conditions.
Treatment regimens
Patients received IFNβ-1a at a dose of 44 or 22 mcg, sc three times weekly for 2 years. To minimize adverse effects, IFNβ-1a was titrated as follows: 8.8 mcg at weeks 1 and 2 of therapy, 22 mcg at weeks 3 and 4, and, for patients treated with the higher dose of IFNβ-1a, 44 mcg from week 5.
Blood sample collection and storage until assay
Blood samples were collected into sterile tubes and allowed to clot spontaneously for 20 minutes at room temperature (i.e., 20-25°C) followed by centrifugation at 3,000 rpm for 10 minutes at 4°C. Sera were immediately aspirated into dry, sterile tubes and stored at -20°C for no longer than 6 months prior to assay. Sera collected for the measurement of neopterin were processed and stored in the dark; sample tubes were covered with aluminum foil throughout the procedure.
Measurement of neopterin, kyn and trp serum levels
All biological parameters were analyzed by an independent laboratory whose personnel was blinded to patients' clinical and treatment information.
• neopterin
Neopterin concentration was measured using a commercially available immunoassay (ELItest, BRAHMS, Berlin, Germany), with a limit of detection of 2 nmol/L. Serum neopterin concentrations in healthy controls were defined as 5.3 ± 2.7 nmol/L, with the upper limit of normal (95th percentile) being 8.7 nmol/L. The assay is a commercial immunoassay which has been reported to be highly reproducible. Coefficients of variation of the assay in our lab are similar to that reported by the manufacturer [i.e. < 5.5% (intra-assay), a < 10.3% (inter-assay)]. The recovery for the neopterin immunoassay was in the range of 91-108%.
• kyn and trp
Serum kyn and trp concentrations were measured by high-performance liquid chromatography. Kyn concentrations were monitored by ultraviolet absorption at 350 nm, while trp was measured by detection of natural fluorescence (excitation wavelength: 285 nm, emission wavelength: 350 nm) [
25,
26] with 3-nitro-L-tyrosine as an internal standard. The coefficient of variation of intra- and interassay determinations for trp and kyn was below 5%. Recovery of trp and kyn was determined by measuring trp and kyn in 20 μl of a pool of 10 sera before and after adding 10 μl of mixture standard solutions of high and low concentration. The recovery for trp and kyn was in the range of 95-105%. Parallel dose-response curves were obtained by serial diluitions of trp and kyn standard solutions and two serially diluted serum samples.
IDO activity was calculated as the ratio of the concentrations of the enzyme product, kyn, divided by its substrate, trp (kyn/trp ratio).
As IDO is not the only enzyme known to trigger the degradation of trp and subsequent kyn production, it was necessary to demonstrate an association between kyn/trp and immune activation using the specific marker, neopterin, in order to confirm IDO involvement.
Measurement of serum Nabs against IFNβ
Measurement of serum NAbs was carried out by an independent laboratory whose personnel was blinded to patients' clinical and treatment information.
A specific training on blood sampling and serum separation was conducted by the Coordinating Center at their lab facilities. A double blood sampling for each measurement was obtained to ensure a full quality control of the analytical procedures.
To detect the presence of NAbs against IFNβ-1a, serum samples were tested by an
antiviral IFNβ neutralization assay that assessed the antiviral activity and its neutralization on the basis of the virus-induced cytopathic effect (CPE). Briefly, monolayers of the human glioblastoma cell line 2D9 were pretreated in 96-well microtiter plates with diluted IFNβ-1a (Rebif
®) preparations (3-10 laboratory units, LU, per ml) that had been pre-incubated for 2 hrs with serial dilutions of the test sera. The cells were then challenged with encephalomyocarditis virus for 24 hrs, stained with 0.05% amido blue black, fixed with 4% formaldehyde in acetic acid buffer and stain was eluted with 0.15 ml of 0.05M NaOH solution before absorbance was read at 620 nm. The NAbs titer was the dilution of serum that reduces 10 LU/ml of IFN to 1 LU/ml (the normal endpoint of antiviral assays). The cut-off for positivity was a titer of 40. Titers were subsequently calculated with the Grossberg-Kawade formula and expressed as ten-fold reducing units (TRU)/ml; cut-off for positivity was 40 TRU/ml [
27,
28].
NAb-positive patients were defined as those presenting positive titers in at least two consecutive valid measurements.
The NAb assay coefficients of variation (intra-assay and inter-assay) never exceed 0.3 Log.
Recovery of NAb assay was determined by measuring NAb titer in 20 μl of a pool of 20 sera before and after adding anti human IFN-beta antibody reference (G038-501-572, National Institute of Health, Bethesda, USA) at high and low concentrations. The recovery for NAb was in the range of 0.3 Log. Parallel line analysis of bioassay showed no significant difference in slopes of dose response curves prepared by serial diluition of human IFNβ antibody reference (G038-501-572) and three serially diluted NAb positive serum samples.
Study approvals
The study was carried out according to the Declaration of Helsinki and its updates, ICH-GCP Guidelines for Clinical Trials and EU Directives. All aspects of the study were discussed with the patients, and each patient gave his/her written informed consent prior to enrollment. The local Ethics Committees approved the study protocol.
Statistical analysis
Data were expressed as means, except for gender that was expressed as percentage (%) and EDSS for which median and standard error (SE) were used.
An Analysis of Variance (ANOVA) for repeated measures was performed to evaluate the effect of time and dose on each of the biological markers. Such an analysis was performed in the entire patient's cohort as well as in sub-groups of patients with or without relapse and patients with or without NAbs.
At each time point, a Mann-Whitney test was performed to identify differences in biological markers and clinical measure between HD and LD groups, between patients with and without clinical relapse and between NAb-positive and NAb-negative patients. Pearson Chi square coefficient was used for comparisons between proportions. Spearman's correlation coefficient was used to evaluate the correlation between laboratory and clinical data.
Discussion
MS is a chronic demyelinating autoimmune disease of the central nervous system (CNS). It is characterized by infiltrates of, mostly, macrophages, T and B lymphocytes, and plasma cells. A variable degree (usually more pronounced in the advanced stages of the disease) of axonal loss and gliotic scars can also be observed. Monocyte-derived macrophages play an important role in these processes and act both as phagocytes and antigen presenting cells (APCs), releasing myelinotoxic factors and proinflammatory cytokines. They are also strongly stimulated by IFNγ secreted by T lymphocytes of the Th1 subset (principal effectors of MS physiopathology).
IFNβ-1a is one of the approved treatments for RRMS patients. The mechanism of actions of IFNβ is still not fully clarified; however, it seems to influence the immune system through an immunomodulatory action and it also enhances the production of several cytokines and proteins [
17].
Validated biological markers of the responsiveness to IFNβ-1a treatment would enable a reliable assessment of the efficacy of MS therapy, both in clinical trials and clinical practice, reducing the need for expensive and time-consuming procedures such as MRI. Such markers, though, have not yet been identified [
29].
Of the several putative candidates, two appeared to us to be particularly promising: neopterin and kyn/trp ratio. The value of both parameters is significantly raised by the action of Th1-secreted-IFNγ on macrophages similarly to reactive oxygen species (ROS), which can be considered as an index of oxidative stress [
30].
Neopterin is a by-product in the synthetic pathway of tetrahydro-biopterin. Upon IFNγ macrophage stimulation, biopterin synthesis is blocked at the step of neopterin whose levels are markedly increased in biological fluids [
3,
31,
32]. Elevated neopterin concentration in body fluids has been observed in a series of conditions characterized by increased Th1 reactivity: infections (particularly HIV), malignancies, autoimmune diseases (particularly RA) and transplants [
33,
34]. Indeed, it can be considered as an indirect indicator of IFNγ levels (difficult to measure
in vivo) and of macrophage stimulation intensity. Neopterin has gained high relevance as a marker of immune activation (Th1 cells) to the point that it is used to monitor patients who received allografts for early detection of possible immunological complications.
In addition, another possible biochemical marker has gained wide acceptance: the enhanced tryptophan degradation induced by IFNγ-stimulated macrophages. Namely, the increased cellular expression and activity of IDO and the ensuing raised N-formyl-kynurenine (a by-product in the biochemical pathway to niacin) levels that are measured in the serum. Tryptophan degradation by IDO (measured as kyn/trp ratio) decreases T lymphocytes proliferation and consequently reduces inflammation and allograft rejection. Hence, a new concept is emerging in immunology: cells expressing IDO can inhibit T cells responses and consequently induce tolerance and reduce inflammation. Therefore, kyn/trp ratio could be regarded as a potential index directly related to treatment efficacy.
This study focused on the evaluation of neopterin levels and kyn/trp ratio as markers of IFNβ biological activity. Out of the 101 INF-naïve RRMS patients enrolled in this study, 78 were fully evaluable after 24 months of IFNβ-1a treatment both for the monitored biomarkers and the clinical variables. In this study, we investigated the dynamic profile of neopterin and kyn/trp ratio and its correlation with the clinical features in patients with RRMS treated with two different doses of IFNβ-1a.
Treatment with IFNβ-1a (both LD and HD) increased serum neopterin levels significantly as compared with pre-treatment levels and a dose-response was evident at each time point (p ≤ 0.046). At month 21 of TP and at the end of the study (month 24) a dose-effect was no longer present since neopterin levels were similar in both treatment groups. This might indicate a similar efficacy, although delayed for the LD group, thus exposing patients treated with the LD to the risk of early relapses in the first months of treatment.
The observed patterns of neopterin production over the 2 years of IFNβ-1a treatment probably reflect a biphasic (short- vs long-term effects) aspect of IFNβ-1a biological activity. Initially, IFNβ-1a administration may result in a sharp increase in the neopterin levels owing to the acute, proinflammatory actions of IFNβ-1a [
35,
36]. However, in the long term its repeated administration may lead to a down-regulation of IFNγ expression and a subsequent decrease in macrophage activation and biomarker expression [
9,
16]. At each time point, the observed effects of IFNβ-1a on neopterin may reflect the relative predominance of short- over long-term effects or vice versa. The increase in biomarker levels in patients receiving the higher dose of IFNβ-1a became less marked with prolonged treatment, possibly due to tachyphylaxis [
19].
A trend showing higher value of kyn/trp ratios in the HD-group was also seen at numerous time points, however, group-differences were not statistically significant at any time point except for month-6 of the TP (p < 0.05). At the end of the study (month 24) a dose-effect was no longer present since kyn/trp ratios were similar in both treatment groups. This finding might indicate that, for tryptophan degradation/IDO activity a ceiling effect might be present at therapeutic dosages.
As previously reported, the increase of kyn/trp ratio in RRMS patients receiving IFNβ-1a indicates the induction of IDO by IFN but such increase does not appear to be dose-dependent [
8]. At present, the impact of IFNβ-1a on tryptophan catabolism in patients with RRMS remains unclear.
As with other proteic drugs, some MS patients develop NAbs against IFNβ, which interfere with the receptor-mediated functions of IFNβ; the clinical relevance of NAbs has been the subject of debate because they appear to decrease treatment efficacy of IFNβ in those patients developing persistent, high titer NAbs [
37]. It has been reported that myxovirus-resistance protein A (MxA), an antiviral protein exclusively induced by type 1 IFNs, is a sensitive measure of the in vivo response to IFNβ and of its reduced activity due to the development of NAbs [
38]. Thus, in the present study, data were also analyzed to determine whether the presence of NAbs affected neopterin serum levels or kyn/trp ratio.
Both, neopterin levels (p = 0.0003) and kyn/trp ratio (p = 0.006) increased over time compared to baseline in each group. Although serum levels of neopterin and kyn/trp ratio at baseline showed no statistical difference between NAb-positive and NAb-negative patients, neopterin levels were significantly reduced in NAb-positive patients starting from month 9 onwards (p < 0.05); the same result was observed for kyn/trp ratio but only at month 9 (p = 0.02). This is a logical consequence of the timing of NAb formation, usually appearing between 3 and 12 months of treatment.
Other studies reported a fall in serum neopterin levels or in the levels of other IFN biologic response markers, including matrix metalloproteinases (MMPs), beta2 microglobulin, MxA, viperin, TNF-related apoptosis-inducing ligand (TRAIL) and X-linked inhibitor apoptosis factor-1 (XAF-1), when NAb titers were elevated in patients with MS [
6,
20,
38‐
41]. Data clearly support the hypothesis that neopterin is a sensitive measure of biological response to IFNβ and is reduced by the presence of NAbs. Nevertheless, since no relations have been found between neopterin and clinical progression, there are issues regarding the use of neopterin as a measure of the clinical efficacy of IFNβ. It is important to underline that, given the nature of MS, a long-term observation would be needed to clearly demonstrate the effects on disease progression, like for MRI. In the present study, the patients analyzed showed a non-NAb-related abrogation of kyn/trp ratio suggesting that the use of the latter as a biological marker of IFNβ treatment may not be predictive of the biological responsiveness to IFNβ.
To gain further insight into the correlation between biomarkers and clinical efficacy, we also investigated whether disease progression and the occurrence of clinical relapses influenced neopterin production and tryptophan degradation.
We found that the presence of disease progression and clinical relapses did not significantly affect biomarker levels. Furthermore, no differences in dose effect were observed between patients who had a clinical worsening during the study period and those who did not, as previously reported [
3,
17]. These findings suggest that, although both biomarkers capture the pharmacodynamic effects of IFNβ-1a, they do not necessarily parallel clinical efficacy. A possible explanation is that the immunoinflammatory process in MS takes place in the CNS and disease activity is only partially reflected in the systemic immune compartment; furthermore, many markers are unstable in the periphery and are rapidly eliminated by the kidneys; therefore, the plasma concentration of many putative markers fluctuate significantly and a single measurement could be a mere snapshot. These observations suggest that probably serum is not the ideal body fluid for measuring this marker concentration in order to monitor disease activity in MS. A further possible explanation is that patients with clinical relapses received high dose intravenous corticosteroids and it appears that this form of treatment can suppress the production of neopterin or tryptophan degradation for a period of time. Regarding disease progression, a later explication of the lack of any correlation between disease progression and biomarker levels variation could be that this is a two years study and does not show the entire clinical course of patients.
Competing interests
The authors declare that they have no competing interests.
Authors' contributions
VD: collected blood samples, performed clinical examination of the patients and wrote the manuscript. AL: collected blood samples, performed clinical examination of the patients and helped to draft the manuscript. PB: collected blood samples and performed clinical examination of the patients. MA: collected blood samples and performed clinical examination of the patients. PB: collected blood samples and performed clinical examination of the patients. GDL: collected blood samples and performed clinical examination of the patients. OP: performed the statistical analysis. RF: collected blood samples and performed clinical examination of the patients. LL: collected blood samples and performed clinical examination of the patients. AS: helped to draft the manuscript. ES: collected blood samples and performed clinical examination of the patients. RT: collected blood samples and performed clinical examination of the patients. SM: collected blood samples and performed clinical examination of the patients. VZ: collected blood samples and performed clinical examination of the patients. MZ: collected blood samples and performed clinical examination of the patients. EM: designed the manuscript.
All authors read and approved the final manuscript.