AI Article Synopsis

  • Fibrosis, caused by excessive scarring after injury, accounts for over 40% of disease-related deaths worldwide and leads to the destruction of organ structure by activated fibroblasts.
  • The study reveals that direct contact with profibrotic macrophages, rather than proinflammatory ones, triggers fibroblast contractions, dependent on specific proteins (αvβ3 integrin and Piezo1).
  • This contact elevates calcium levels in fibroblasts, activating transcription factors that drive fibroblast activation, suggesting that targeting the mechanisms of macrophage-fibroblast interaction could help develop antifibrosis treatments.

Article Abstract

Fibrosis-excessive scarring after injury-causes >40% of disease-related deaths worldwide. In this misguided repair process, activated fibroblasts drive the destruction of organ architecture by accumulating and contracting extracellular matrix. The resulting stiff scar tissue, in turn, enhances fibroblast contraction-bearing the question of how this positive feedback loop begins. We show that direct contact with profibrotic but not proinflammatory macrophages triggers acute fibroblast contractions. The contractile response depends on αvβ3 integrin expression on macrophages and Piezo1 expression on fibroblasts. The touch of macrophages elevates fibroblast cytosolic calcium within seconds, followed by translocation of the transcription cofactors nuclear factor of activated T cells 1 and Yes-associated protein, which drive fibroblast activation within hours. Intriguingly, macrophages induce mechanical stress in fibroblasts on soft matrix that alone suppresses their spontaneous activation. We propose that acute contact with suitable macrophages mechanically kick-starts fibroblast activation in an otherwise nonpermissive soft environment. The molecular components mediating macrophage-fibroblast mechanotransduction are potential targets for antifibrosis strategies.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11498225PMC
http://dx.doi.org/10.1126/sciadv.adp4726DOI Listing

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