A rapid and efficient method for neuronal induction of the P19 embryonic carcinoma cell line

Yoshiaki Nakayama; Ayumi Wada; Rei Inoue; Kazuya Terasawa; Ikuo Kimura; Naosuke Nakamura; Akira Kurosaka

doi:10.1016/j.jneumeth.2014.02.011

A rapid and efficient method for neuronal induction of the P19 embryonic carcinoma cell line

J Neurosci Methods. 2014 Apr 30:227:100-6. doi: 10.1016/j.jneumeth.2014.02.011. Epub 2014 Feb 28.

Authors

Yoshiaki Nakayama¹, Ayumi Wada¹, Rei Inoue¹, Kazuya Terasawa², Ikuo Kimura³, Naosuke Nakamura¹, Akira Kurosaka⁴

Affiliations

¹ Laboratory of Neuroglycobiology, Department of Molecular Sciences, Faculty of Life Sciences, Kyoto Sangyo University, Kamigamo-motoyama, Kita-ku, Kyoto 603-8555, Japan.
² Center for Genomics Medicine, Kyoto University Graduate School of Medicine, Sakyo-ku, Kyoto 606-8507, Japan.
³ Department of Pharmacogenomics, Kyoto University Graduate School of Pharmaceutical Science, Sakyo-ku, Kyoto 606-8501, Japan; Department of Applied Biological Science, Tokyo University of Agriculture and Technology, Fuchu-city, Tokyo 183-8538, Japan.
⁴ Laboratory of Neuroglycobiology, Department of Molecular Sciences, Faculty of Life Sciences, Kyoto Sangyo University, Kamigamo-motoyama, Kita-ku, Kyoto 603-8555, Japan. Electronic address: kurosaka@cc.kyoto-su.ac.jp.

PMID: 24583076
DOI: 10.1016/j.jneumeth.2014.02.011

Abstract

Background: P19 mouse embryonic carcinoma cells are conventionally induced to differentiate into neural cells by suspension culture in the presence of retinoic acid to form cell aggregates, followed by adhesion culture in a poly-l-lysine-coated dish. Drawbacks of this procedure include it taking more than 10 days to obtain mature neurons, and non-neuronal proliferating cells occupying the majority of the cell population with time.

New method: Here, we show a novel method for the rapid and efficient neurogenesis of P19 cells, without aggregate formation in a suspension culture. The new approach is based on an adherent serum-free culture in a laminin-coated dish in the presence of FGF8, a γ-secretase inhibitor, and cytosine arabinoside.

Results: The new method efficiently induced P19 cells to differentiate into neurons within 4 days, and subsequently into mature neurons that were responsive to several neurotransmitters, giving spontaneous neuronal network activity within 6 days.

Comparison with existing method: The novel method accelerated neuritogenesis and enhanced population of neuron selectively compared to the conventional method. Proliferating non-neuronal cells were eliminated by adding cytosine arabinoside during neuronal maturation.

Conclusions: The method is useful for studying neuronal differentiation or activities.

Keywords: Neural differentiation; Neurotransmitter; P19 cells.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Calcium / metabolism
Carcinoma, Embryonal / pathology
Cell Culture Techniques / methods
Cell Differentiation / physiology*
Cell Line, Tumor
Culture Media, Serum-Free / pharmacology
Fibroblast Growth Factor 8 / pharmacology
Gene Expression Regulation, Neoplastic / drug effects
Gene Expression Regulation, Neoplastic / physiology
Laminin / metabolism
Laminin / pharmacology
Mice
Nerve Tissue Proteins / genetics
Nerve Tissue Proteins / metabolism
Neurogenesis / drug effects
Neurogenesis / physiology*
Neurons / physiology*
Neurotransmitter Agents / pharmacology
Potassium Chloride / pharmacology
Time Factors

Substances

Culture Media, Serum-Free
Fgf8 protein, mouse
Laminin
Nerve Tissue Proteins
Neurotransmitter Agents
Fibroblast Growth Factor 8
Potassium Chloride
Calcium