4.8 Article

Increased connectivity of hiPSC-derived neural networks in multiphase granular hydrogel scaffolds

期刊

BIOACTIVE MATERIALS
卷 9, 期 -, 页码 358-372

出版社

KEAI PUBLISHING LTD
DOI: 10.1016/j.bioactmat.2021.07.008

关键词

Microgel; Hydrogel; Hyaluronan; iPSC; Neural tissue engineering; 3D printing

资金

  1. Biotechnology and Biological Sciences Research Council [BB/H008527/1]
  2. China Regenerative Medicine International (CRMI)
  3. Jiangsu Industrial Technology Research Institute (JITRI)
  4. Engineering and Physical Sciences Research Council (EPSRC) [EP/P005381/1, EP/V007785/1]

向作者/读者索取更多资源

The study successfully supported 3D hiPSC-derived neural networks using granular hydrogel-based scaffolds, resulting in improved cell viability and longer neurite extensions. This method is simple, rapid, and efficient, achieving tissue-relevant granular structures in hydrogel cultures.
To reflect human development, it is critical to create a substrate that can support long-term cell survival, differentiation, and maturation. Hydrogels are promising materials for 3D cultures. However, a bulk structure consisting of dense polymer networks often leads to suboptimal microenvironments that impedes nutrient exchange and cell-to-cell interaction. Herein, granular hydrogel-based scaffolds were used to support 3D human induced pluripotent stem cell (hiPSC)-derived neural networks. A custom designed 3D printed toolset was developed to extrude hyaluronic acid hydrogel through a porous nylon fabric to generate hydrogel granules. Cells and hydrogel granules were combined using a weaker secondary gelation step, forming self-supporting cell laden scaffolds. At three and seven days, granular scaffolds supported higher cell viability compared to bulk hydrogels, whereas granular scaffolds supported more neurite bearing cells and longer neurite extensions (65.52 +/- 11.59 mu m) after seven days compared to bulk hydrogels (22.90 +/- 4.70 mu m). Long-term (three-month) cultures of clinically relevant hiPSC-derived neural cells in granular hydrogels supported well established neuronal and astrocytic colonies and a high level of neurite extension both inside and beyond the scaffold. This approach is significant as it provides a simple, rapid and efficient way to achieve a tissue-relevant granular structure within hydrogel cultures.

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