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Improvements in in vitro spermatogenesis: oxygen concentration, antioxidants, tissue-form design, and space control. | LitMetric

AI Article Synopsis

  • The study explored using a basic culture medium, MEMα, with bovine serum albumin (AlbuMAX) for in vitro spermatogenesis in mice but found it ineffective in other animals, prompting a search for alternatives.
  • Researchers identified essential components for a synthetic culture medium that promotes spermatogenesis, including antioxidants and lysophospholipids, in addition to known factors like retinoic acid and hormones.
  • They developed a new technique called the PDMS-ceiling method to optimize nutrient and oxygen supply, successfully achieving in vitro spermatogenesis in rats, which previously posed challenges, and aim to improve conditions for other animal species.

Article Abstract

Incorporation of bovine serum-derived albumin formulation (AlbuMAX) into a basic culture medium, MEMα, enables the completion of in vitro spermatogenesis through testicular tissue culture in mice. However, this medium was not effective in other animals. Therefore, we sought an alternative approach for in vitro spermatogenesis using a synthetic medium without AlbuMAX and aimed to identify its essential components. In addition to factors known to be important for spermatogenesis, such as retinoic acid and reproductive hormones, we found that antioxidants (vitamin E, vitamin C, and glutathione) and lysophospholipids are vital for in vitro spermatogenesis. Moreover, based on our experience with microfluidic devices (MFD), we developed an alternative approach, the PDMS-ceiling method (PC method), which involves simply covering the tissue with a flat chip made of PDMS, a silicone resin material used in MFD. The PC method, while straightforward, integrates the advantages of MFD, enabling improved and uniform oxygen and nutrient supply via tissue flattening. Furthermore, our studies underscored the significance of lowering the oxygen concentration to 10-15%. Using an integrated cultivation method based on these findings, we successfully achieved in vitro spermatogenesis in rats, which has been a long-standing challenge. Further improvements in culture conditions would pave the way for spermatogenesis completion in diverse animal species.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10902634PMC
http://dx.doi.org/10.1262/jrd.2023-093DOI Listing

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