National Psoriasis Foundation - Dendritic Cell-Specific Transmembrane Protein (DC-Stamp) Biomarker Study

University of Rochester22 enrolled

Overview

The purpose of this study is to determine whether DC-STAMP, a protein on the surface of osteoclast precursors (OCPs), can be used as a biologic marker in Psoriatic Arthritis (PsA). With this marker the investigators hope to learn more about how OCPs develop as well as find out if DC-STAMP predicts PsA severity and how well treatment works in PsA.

Psoriatic Arthritis (PsA), a phenotypically heterogeneous disorder, is characterized by joint damage observed in over half of the patients with early disease. While anti-tumor necrosis factor (TNF) agents have greatly improved signs and symptoms and lessened joint damage, the fact that only a fraction of patients achieve complete remission underscores the tremendous unmet need for this population. To date, a biomarker that can stratify patients by severity and can serve as a leading indicator of treatment response has not been identified. Our laboratory demonstrated that circulating osteoclast precursors (OCP) are elevated in PsA patients. OCP decline rapidly following anti-TNF therapy and levels are higher in subjects with erosive arthritis compared to those with no x-ray changes. The OCP are derived from CD14+ monocytes and the assay entails culture techniques that are costly, expensive and labor intensive. We developed an antibody (1A2) to Dendritic Cell Specific Transmembrane Protein (DC-STAMP), a potential marker of the OCP population, for analysis by flow cytometry. We found that: 1) the level of monocyte DC-STAMP expression correlated with in vitro osteoclast formation; 2) DC-STAMP expression is significantly elevated in PBMC from PsA subjects compared to controls; 3) TNF dramatically upregulated the expression of DC-STAMP in vitro; 4) DC-STAMP surface expression declined following anti-TNF therapy; 5) subsets of CD3+ cells also express DC-STAMP on the cell membrane. Based on these preliminary data, three hypotheses are proposed: 1. DC-STAMP+ CD3+ T cells belong to the Th17 subset which facilitates OC generation; 2. DC-STAMP is a marker of disease severity in PsA; 3. DC-STAMP is a biomarker of treatment response in PsA. We propose three Specific Aims to test these hypotheses. Aim 1 To examine whether DC-STAMP+CD3+ cells belong to the Th17 cell subset, PBMC will be stained with Th17-specific antibodies in PsA subjects with elevated DC-STAMP expression. We will also examine the role of T cells in osteoclastogenesis directly by co-culture experiments and we will use monocyte cultures without added lymphocytes as controls. The expression of DC-STAMP on circulating dendritic cells will be examined ex vivo with 11-color flow cytometry. Aim 2 To determine if increased DC-STAMP expression is associated with more severe features of PsA, DC-STAMP expression in 40 PsA subjects will be determined and correlated with clinical variables of arthritis and skin disease, CRP and x-ray damage. Aim 3 To examine if DC-STAMP is a response marker to anti-TNF treatment, we will recruit 20 PsA patients in Aim 2 with elevated DC-STAMP expression and divide them into 2 groups. Ten subjects will receive methotrexate, and ten will receive anti-TNF therapy. The correlation between DC-STAMP variables (percentage of 1A2+ divided by 1A2 - cells X 100) and the variables detailed in Aim 2 will be analyzed in these 2 treatment groups at 2 different time points.

Study Type

OBSERVATIONAL

Enrollment

Conditions

Psoriatic Arthritis

Interventions

MethotrexateDRUG

Subjects will start Methotrexate which will be escalated from 7.5 mg weekly to 15 mg/weekly over a 3 week period.

Anti-TNFDRUG

Anti-TNF to be administered per standard of care within the practice.

Eligibility

Sex: ALLMin age: 18 Years

Medical Language ↔ Plain English

Inclusion Criteria: 1. Subject must be \>18 years old 2. Subject must have \>3 tender and swollen joints 3. Subject must have must have a target lesion of greater than 3 cm in diameter 4. Subjects who meet the the ClASsification of Psoriatic ARthritis (CASPAR) criteria for PsA 5. Subjects must have a DC-STAMP pattern III or IV Exclusion Criteria: 1. Subjects with active inflammatory synovitis, dactylitis, enthesitis, osteoarthritis, axial disease, Subjects with a SLE, Sjogren's syndrome, scleroderma or inflammatory muscle disease 2. Subjects with an active malignancy 3. Subjects currently on biologic agents (anti-TNF agents, anti-T or B cells agents) and/or disease-modifying antirheumatic drugs (DMARDs) (methotrexate, leflunomide, hydroxychloroquine, azulfidine, cyclosporine, azathioprine) 4. Subjects who have been off DMARDs or biologics for less than 3 months 5. Subjects judged ineligible at the discretion of the PI 6. Subjects with a history of crystalline arthritis (gout, pseudogout) 7. Subject pregnancy or breast feeding 8. History of recurrent infections - AIM 3 Specific 9. Demyelinating disorders - AIM 3 Specific 10. Prior non-responsiveness to TNFi - AIM 3 Specific 11. Subjects who have a BMI \>30 - AIM 3 Specific MTX arm 12. Subjects who have a history of type II diabetes - AIM 3 Specific MTX arm 13. Subjects with a history of substance abuse including alcohol - AIM 3 Specific MTX arm

Locations (1)

University of Rochester

Rochester, New York, United States

Outcomes

Primary Outcomes

Analysis of T cell subset and dendritic cell (DC) subset for DC-STAMP expression

Determine whether DC-STAMP+ cells belong to the Th17 subset and also analyze the DC subsets for DC-STAMP expression.

Time frame: Week 0 (Baseline)

Analysis of T cell subset and DC subset for DC-STAMP expression

Determine whether DC-STAMP+ cells belong to the Th17 subset and also analyze the DC subsets for DC-STAMP expression.

Time frame: Week 16

DC-STAMP as a marker of disease severity in PsA

Baseline measurement of DC-STAMP expression will be collected in order to assist in determining whether it is associated with more severe features of PsA. DC-STAMP expression will be correlated with clinical variables of arthritis and skin disease, CRP and x-ray damage.

Time frame: Week 0 (Baseline)

DC-STAMP as a marker of disease severity in PsA

Measurement of DC-STAMP expression will be collected in order to assist in determining whether it is associated with more severe features of PsA. DC-STAMP expression will be correlated with clinical variables of arthritis and skin disease, CRP and x-ray damage.

Time frame: Week 16

DC-STAMP as a biomarker of treatment response in PsA

A baseline measurement of DC-STAMP as a response marker to treatment will be collected. Ten subjects will receive methotrexate and ten will receive anti-TNF therapy. The correlation between DC-STAMP variables (percentage of 1A2+ divided by 1A2 - cells X 100) and the variables detailed in Aim 2 will be analyzed in these 2 treatment groups at 2 different time points.

Time frame: Week 0 (Baseline)

DC-STAMP as a biomarker of treatment response in PsA

A measurement of DC-STAMP as a response marker to treatment will be collected. Ten subjects received methotrexate and ten received anti-TNF therapy. The correlation between DC-STAMP variables (percentage of 1A2+ divided by 1A2 - cells X 100) and the variables detailed in Aim 2 will be analyzed in these 2 treatment groups at 2 different time points.

Data from ClinicalTrials.gov

This platform is for informational purposes only and does not constitute medical advice. Always consult a qualified healthcare professional.