High-throughput screening discovers antifibrotic properties of haloperidol by hindering myofibroblast activation
Michael Rehman, Simone Vodret, Luca Braga, Corrado Guarnaccia, Fulvio Celsi, Giulia Rossetti, Valentina Martinelli, Tiziana Battini, Carlin Long, Kristina Vukusic, Tea Kocijan, Chiara Collesi, Nadja Ring, Natasa Skoko, Mauro Giacca, Giannino Del Sal, Marco Confalonieri, Marcello Raspa, Alessandro Marcello, Michael P. Myers, Sergio Crovella, Paolo Carloni, Serena Zacchigna
Michael Rehman, Simone Vodret, Luca Braga, Corrado Guarnaccia, Fulvio Celsi, Giulia Rossetti, Valentina Martinelli, Tiziana Battini, Carlin Long, Kristina Vukusic, Tea Kocijan, Chiara Collesi, Nadja Ring, Natasa Skoko, Mauro Giacca, Giannino Del Sal, Marco Confalonieri, Marcello Raspa, Alessandro Marcello, Michael P. Myers, Sergio Crovella, Paolo Carloni, Serena Zacchigna
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Research Article Cell biology Pulmonology

High-throughput screening discovers antifibrotic properties of haloperidol by hindering myofibroblast activation

Abstract

Fibrosis is a hallmark in the pathogenesis of various diseases, with very limited therapeutic solutions. A key event in the fibrotic process is the expression of contractile proteins, including α-smooth muscle actin (αSMA) by fibroblasts, which become myofibroblasts. Here, we report the results of a high-throughput screening of a library of approved drugs that led to the discovery of haloperidol, a common antipsychotic drug, as a potent inhibitor of myofibroblast activation. We show that haloperidol exerts its antifibrotic effect on primary murine and human fibroblasts by binding to sigma receptor 1, independent from the canonical transforming growth factor-β signaling pathway. Its mechanism of action involves the modulation of intracellular calcium, with moderate induction of endoplasmic reticulum stress response, which in turn abrogates Notch1 signaling and the consequent expression of its targets, including αSMA. Importantly, haloperidol also reduced the fibrotic burden in 3 different animal models of lung, cardiac, and tumor-associated fibrosis, thus supporting the repurposing of this drug for the treatment of fibrotic conditions.

Authors

Michael Rehman, Simone Vodret, Luca Braga, Corrado Guarnaccia, Fulvio Celsi, Giulia Rossetti, Valentina Martinelli, Tiziana Battini, Carlin Long, Kristina Vukusic, Tea Kocijan, Chiara Collesi, Nadja Ring, Natasa Skoko, Mauro Giacca, Giannino Del Sal, Marco Confalonieri, Marcello Raspa, Alessandro Marcello, Michael P. Myers, Sergio Crovella, Paolo Carloni, Serena Zacchigna

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Figure 1

High-throughput screening identifies several modulators of αSMA expression in myofibroblasts.

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High-throughput screening identifies several modulators of αSMA expressi...
(A) Pie chart showing the main categories of the 640 FDA-approved drugs included in the library. (B) Results of the high-throughput screening shown as the Z score of the αSMA mean cellular intensity in αSMA-RFP/CoLL-EGFP fibroblasts, treated with each drug at 48 hours of culture. Top hits upregulating αSMA expression are indicated in red, whereas those downregulating αSMA expression are indicated in green. (C) Representative images of αSMA-RFP/COLL-EGFP fibroblasts exposed to the indicated drugs (abbreviations are explained in panel B). Green fluorescence indicates collagen expression (COLL-EGFP), whereas red fluorescence indicates αSMA expression (αSMA-RFP). Nuclei are stained blue with Hoechst. (D) Cardiac fibroblasts treated with TGF-β alone and in combination with various drugs, stained red with anti-αSMA antibodies. Nuclei are stained blue with Hoechst. The chemical structure of each drug is shown under the corresponding cell picture. Atom color assignment: gray, carbon; red, oxygen; green, halogen; blue, nitrogen; orange, phosphorus; purple, sodium. (E) Quantification of the αSMA mean fluorescence intensity upon treatment with TGF-β alone and in combination with the indicated drugs (n = 3/gp). (F) Western blot showing the expression of αSMA in primary cardiac fibroblasts treated with TGF-β, haloperidol (3 μM), or their combination. Actin is shown as loading control. (G) Quantification of αSMA levels in primary cardiac fibroblasts treated with TGF-β, haloperidol (3 μM), and their combination (n = 4/gp). (H) Expression levels of Col1a1, Fn1, Postn, and Acta2 upon treatment with TGF-β, haloperidol, and their combination (n = 3/gp). Values in E, G, and H are mean ± SEM. *P < 0.05, **P < 0.01, ***P < 0.001 by unpaired t test with Welch’s correction. Scale bars in C and D: 50 μm.