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Melatonin Increases Collagen Content Accumulation and Fibroblast Growth Factor-2 Secretion in Cultured Human Cardiac Fibroblasts.

Marta Drobnik, Agnieszka Tomaszewska, Joanna Ryżko, Aleksandra Kędzia,Małgorzata Gałdyszyńska,Lucyna Piera, Justyna Rydel,Jacek Szymański,Jacek Drobnik

Pharmacological Reports(2023)

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摘要
The extracellular matrix serves as a scaffold for cardiomyocytes, allowing them to work in accord. In rats, collagen metabolism within a myocardial infarction scar is regulated by melatonin. The present study determines whether melatonin influences matrix metabolism within human cardiac fibroblast cultures and examines the underlying mechanism. The experiments were performed on cultures of cardiac fibroblasts. The Woessner method, 1,9-dimethylmethylene blue assay, enzyme-linked immunosorbent assay and quantitative PCR were used in the study. Melatonin treatment lowered the total cell count within the culture, elevated necrotic and apoptotic cell count as well as augmented cardiac fibroblast proliferation, and increased total, intracellular, and extracellular collagen within the fibroblast culture; it also elevated type III procollagen α1 chain expression, without increasing procollagen type I mRNA production. The pineal hormone did not influence matrix metalloproteinase-2 (MMP-2) release or glycosaminoglycan accumulation by cardiac fibroblasts. Melatonin increased the release of Fibroblast Growth Factor-2 (FGF-2) by human cardiac fibroblasts, but cardiotrophin release was not influenced. Within human cardiac fibroblast culture, collagen metabolism is regulated by melatonin. The profibrotic effect of melatonin depends on the elevation of procollagen type III gene expression, and this could be modified by FGF-2. Two parallel processes, viz., cell elimination and proliferation, induced by melatonin, lead to excessive replacement of cardiac fibroblasts.
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关键词
Cell cultures,Collagen,Connective tissue,Fibroblast,Glycosaminoglycan,Heart,Melatonin,Proliferation
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