Cysteine-rich domain of type III collagen N-propeptide inhibits fibroblast activation by attenuating TGFβ signaling

成纤维细胞 化学 肌成纤维细胞 细胞外基质 细胞生物学 转化生长因子 真皮成纤维细胞 信号转导 癌症研究 内科学 生物 纤维化 生物化学 医学 体外
作者
Becky K. Brisson,Daniel Stewart,Chelsea M. Burgwin,David M. Chenoweth,Rebecca G. Wells,Sherrill Adams,Susan W. Volk
出处
期刊:Matrix Biology [Elsevier BV]
卷期号:109: 19-33 被引量:21
标识
DOI:10.1016/j.matbio.2022.03.004
摘要

• A novel regulatory role for a cysteine-rich domain of Type III collagen was examined • CR peptide binds to TGFβ with high affinity and in a dose dependent manner • The CR peptide attenuates TGFβ signaling in fibroblasts and breast cancer cells • CR peptide tempers myofibroblast activation and function • In vivo studies support CR's potential to control scarring, fibrosis and tumor activities TGFβ is a key regulator of the dynamic reciprocity between cells and the extracellular matrix that drives physiologic and pathologic responses in both tissue repair and tumor microenvironments. Our studies define type III Collagen (Col3) as a suppressor of scar formation and desmoplasia through its effects, in part, on myofibroblasts. TGFβ stimulates activation of myofibroblasts, and here, we demonstrate that cultured Col3-deficient fibroblasts have increased TGFβ signaling compared to wild-type fibroblasts. Moreover, kinetic binding studies show that a synthetic peptide containing a Col3 cysteine-rich (CR) domain found within its N-propeptide binds in a dose-dependent manner to TGFβ1, while a CR control peptide with mutated cysteines does not, suggesting that Col3 attenuates TGFβ signaling in part through the N-propeptide CR domain. Consistent with this hypothesis, the CR peptide attenuates TGFβ signaling in fibroblasts and 4T1 breast cancer cells and suppresses fibroblast activation and contraction, as assessed by α-smooth-muscle actin staining, cell wrinkling of deformable silicone, and stressed-fibroblast populated collagen lattice contraction assays. Finally, CR peptide treatment of orthotopically injected breast cancer cells (4T1) suppresses intratumoral fibroblast activation and inhibits primary tumor growth compared to CR control. Treatment with the CR peptide decreases both intratumoral canonical and non-canonical downstream TGFβ signaling targets, consistent with its extracellular binding to TGFβ. Taken together, our results suggest that the Col3 N-propeptide CR domain binds TGFβ1 and attenuates (but importantly does not eliminate) TGFβ signaling in fibroblasts and cancer cells. Expanding on our previous work, this study demonstrates an additional mechanism by which Col3 regulates cell behaviors in post-injury and tumor microenvironments and suggests that novel Col3-targeted strategies could effectively control biologic responses in vivo and improve anti-scarring/fibrosis and oncologic therapies.
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