Stimulatory Effect of Tofacitinib on Bone Marrow Adipocytes Differentiation

Jean-Guillaume Letarouilly; Julien Paccou; Sammy Badr; Christophe Chauveau; Odile Broux; Aline Clabaut

doi:10.3389/fendo.2022.881699

Stimulatory Effect of Tofacitinib on Bone Marrow Adipocytes Differentiation

Front Endocrinol (Lausanne). 2022 Jul 6:13:881699. doi: 10.3389/fendo.2022.881699. eCollection 2022.

Authors

Jean-Guillaume Letarouilly¹, Julien Paccou¹, Sammy Badr², Christophe Chauveau³, Odile Broux³, Aline Clabaut³

Affiliations

¹ Université de Lille, Centre Hospitalier Universitaire CHU CENTRE HOSPITALIER UNIVERSITAIRE (CHU) Lille, MABLab ULR 4490, Service de Rhumatologie, Lille, France.
² Université de Lille, Centre Hospitalier Universitaire (CHU) Lille, MABLab ULR 4490, Service de Radiologie et Imagerie Musculosquelettique, Lille, France.
³ Université Littoral Côte d'Opale, MABLab ULR 4490, Boulogne-sur-Mer, France.

Abstract

Background: Systemic inflammation is the main factor underlying secondary osteoporosis in patients with rheumatoid arthritis (RA). Janus kinase inhibitors (JAKi), such as tofacitinib (Tofa), can control systemic inflammation and may have beneficial effects on bone in various models. This might be due to direct effects on the bone microenvironment and not exclusively based on their anti-inflammatory function. Bone marrow adipocytes (BMAds) are abundant in the bone microenvironment. The effect of JAKi on BMAds is unknown, but evidence suggests that there is competition between human bone marrow-derived stromal cell (hBMSC) differentiation routes towards BMAds and osteoblasts (Ob) in osteoporosis.

Objectives: The aims of the study are to determine whether Tofa influences BMAds and Ob derived from hBMSCs and to investigate the potential effects of Tofa on bone marrow adiposity in RA patients.

Methods: To determine the effect of Tofa on cellular commitment, hBMSCs were differentiated to BMAds or OBs for 3 days together with Tofa at 200, 400, or 800 nM and TNFα. This study was also conducted using differentiated BMAds. The impact of Tofa was determined by gene and protein expression analysis and cell density monitoring. In parallel, in a pilot study of 9 RA patients treated with Tofa 5 mg twice a day (NCT04175886), the proton density fat fraction (PDFF) was measured using MRI at the lumbar spine at baseline and at 6 months.

Results: In non-inflammatory conditions, the gene expression of Runx2 and Dlx5 decreased in Ob treated with Tofa (p <0.05). The gene expression of PPARγ2, C/EBPα, and Perilipin 1 were increased compared to controls (p <0.05) in BMAds treated with Tofa. Under inflammatory conditions, Tofa did not change the expression profiles of Ob compared to TNFα controls. In contrast, Tofa limited the negative effect of TNFα on BMAd differentiation (p <0.05). An increase in the density of differentiated BMAds treated with Tofa under TNFα was noted (p <0.001). These findings were consolidated by an increase in PDFF at 6 months of treatment with Tofa in RA patients (46.3 ± 7.0% versus 53.2 ± 9.2% p <0.01).

Conclusion: Together, these results suggest a stimulatory effect of Tofa on BMAd commitment and differentiation, which does not support a positive effect of Tofa on bone.

Keywords: bone marrow adipocytes; differentiation; human bone marrow-derived stromal cells; osteoblasts; rheumatoid arthritis; tofacitinib.

MeSH terms

Adipocytes / metabolism
Arthritis, Rheumatoid* / complications
Arthritis, Rheumatoid* / drug therapy
Arthritis, Rheumatoid* / metabolism
Bone Marrow
Clinical Studies as Topic
Humans
Inflammation / metabolism
Osteoporosis* / metabolism
Pilot Projects
Piperidines
Pyrimidines

Substances

Piperidines
Pyrimidines
tofacitinib

Associated data

ClinicalTrials.gov/NCT04175886