PLoS ONE (Jan 2009)

Self-contained induction of neurons from human embryonic stem cells.

  • Tsuyoshi Okuno,
  • Takashi Nakayama,
  • Nae Konishi,
  • Hideo Michibata,
  • Koji Wakimoto,
  • Yutaka Suzuki,
  • Shinji Nito,
  • Toshio Inaba,
  • Imaharu Nakano,
  • Shin-Ichi Muramatsu,
  • Makoto Takano,
  • Yasushi Kondo,
  • Nobuo Inoue

DOI
https://doi.org/10.1371/journal.pone.0006318
Journal volume & issue
Vol. 4, no. 7
p. e6318

Abstract

Read online

BACKGROUND: Neurons and glial cells can be efficiently induced from mouse embryonic stem (ES) cells in a conditioned medium collected from rat primary-cultured astrocytes (P-ACM). However, the use of rodent primary cells for clinical applications may be hampered by limited supply and risk of contamination with xeno-proteins. METHODOLOGY/PRINCIPAL FINDINGS: We have developed an alternative method for unimpeded production of human neurons under xeno-free conditions. Initially, neural stem cells in sphere-like clusters were induced from human ES (hES) cells after being cultured in P-ACM under free-floating conditions. The resultant neural stem cells could circumferentially proliferate under subsequent adhesive culture, and selectively differentiate into neurons or astrocytes by changing the medium to P-ACM or G5, respectively. These hES cell-derived neurons and astrocytes could procure functions similar to those of primary cells. Interestingly, a conditioned medium obtained from the hES cell-derived astrocytes (ES-ACM) could successfully be used to substitute P-ACM for induction of neurons. Neurons made by this method could survive in mice brain after xeno-transplantation. CONCLUSION/SIGNIFICANCE: By inducing astrocytes from hES cells in a chemically defined medium, we could produce human neurons without the use of P-ACM. This self-serving method provides an unlimited source of human neural cells and may facilitate clinical applications of hES cells for neurological diseases.