AI Article Synopsis

  • Connective tissue models derived from cell monolayers are valuable for drug screening, wound healing, and regenerative engineering, but they struggle to assemble and maintain fibrillar collagen like in the body.
  • The use of macromolecular crowding (MMC) has proven effective in enhancing fibrillar collagen assembly and accumulation in cell cultures.
  • This study combined carrageenan hydrogel to release soluble macromolecules and act as a confinement barrier, which improved collagen accumulation in human MG-63 bone cells without affecting cell viability.

Article Abstract

Connective tissue models grown from cell monolayers can be instrumental in a variety of biomedical fields such as drug screening, wound healing, and regenerative engineering. However, while connective tissues contain abundant fibrillar collagen, achieving a sufficient assembly and retention of fibrillar collagen in vitro is challenging. Unlike the dilute cell culture environment, the body's environment is characterized by a high density of soluble macromolecules (crowding) and macromolecular networks (confinement), which contribute to extracellular matrix (ECM) assembly in vivo. Consequently, macromolecular crowding (MMC) has been successfully used to enhance the processing of type I procollagen, leading to significant increases in fibrillar collagen assembly and accumulation during in vitro culture of a variety of cell types. In this study, we developed a combination approach using a carrageenan hydrogel, which released soluble macromolecules and served as a confinement barrier. We first evaluated the local carrageenan release and then confirmed the effectiveness of this combination approach on collagen accumulation by the human MG-63 bone cell line. Additionally, computational modeling of oxygen and glucose transport within the culture system showed no negative effects of the hydrogel and its releasates on cell viability.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10529090PMC
http://dx.doi.org/10.3390/gels9090705DOI Listing

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