Oxidative stress promotes fibrosis in systemic sclerosis through stabilization of a kinase-phosphatase complex
Ruiyuan Zhang, … , Wolfgang Peti, Nunzio Bottini
Ruiyuan Zhang, … , Wolfgang Peti, Nunzio Bottini
Published April 22, 2022
Citation Information: JCI Insight. 2022;7(8):e155761. https://doi.org/10.1172/jci.insight.155761.
View: Text | PDF
Research Article Inflammation

Oxidative stress promotes fibrosis in systemic sclerosis through stabilization of a kinase-phosphatase complex

Abstract

Systemic sclerosis (SSc) is a fibrotic autoimmune disease characterized by pathogenic activation of fibroblasts enhanced by local oxidative stress. The tyrosine phosphatase PTP4A1 was identified as a critical promoter of TGF-β signaling in SSc. Oxidative stress is known to functionally inactivate tyrosine phosphatases. Here, we assessed whether oxidation of PTP4A1 modulates its profibrotic action and found that PTP4A1 forms a complex with the kinase SRC in scleroderma fibroblasts, but surprisingly, oxidative stress enhanced rather than reduced PTP4A1’s association with SRC and its profibrotic action. Through structural assessment of the oxo-PTP4A1-SRC complex, we unraveled an unexpected mechanism whereby oxidation of a tyrosine phosphatase promotes its function through modification of its protein complex. Considering the importance of oxidative stress in the pathogenesis of SSc and fibrosis, our findings suggest routes for leveraging PTP4A1 oxidation as a potential strategy for developing antifibrotic agents.

Authors

Ruiyuan Zhang, Ganesan Senthil Kumar, Uwe Hansen, Martina Zoccheddu, Cristiano Sacchetti, Zachary J. Holmes, Megan C. Lee, Denise Beckmann, Yutao Wen, Zbigniew Mikulski, Shen Yang, Eugenio Santelli, Rebecca Page, Francesco Boin, Wolfgang Peti, Nunzio Bottini

×

Figure 2

Oxidative stress promotes PTP4A1 and SRC association.

Options: View larger image (or click on image) Download as PowerPoint
Oxidative stress promotes PTP4A1 and SRC association. (A) Representative...
(A) Representative PTP4A1-SRC PLA signal in TGF-β–stimulated SScDFs treated with or without NAC (left) with quantification (right). n = 8 experiments across 7 cell lines. (B) Representative Western blotting image of co-IP between PTP4A1 and SRC from HEK293T cells untreated or incubated with H2O2 (top) with quantification (bottom). n = 5, reducing buffer. Rabbit IgG was used for control IP. (C) Binding of SRC to Ni-NTA agarose-bound His6-tagged oxidized/reduced PTP4A1. Ni-NTA agarose beads were used as control. Non-reducing buffer. (A) Blue = DAPI, magenta = PLA. (A) Images were captured with 40× original magnification. Data shown are mean ± SEM of data normalized to the control averages. Two-tailed paired t test from the non-normalized data in A, 2-tailed Welch’s t test in B, 1-way ANOVA in C. **P < 0.01, ***P < 0.001.