Healthy human CSF promotes glial differentiation of hESC-derived neural cells while retaining spontaneous activity in existing neuronal networks

Author:

Kiiski Heikki12,Äänismaa Riikka2,Tenhunen Jyrki13,Hagman Sanna4,Ylä-Outinen Laura2,Aho Antti5,Yli-Hankala Arvi6,Bendel Stepani7,Skottman Heli8,Narkilahti Susanna29

Affiliation:

1. Critical Care Medicine Research Group, Department of Intensive Care Unit, Tampere University Hospital, FI-33521 Tampere, Finland

2. NeuroGroup, Institute of Biomedical Technology/BioMediTech, University of Tampere, FI-33520 Tampere, Finland

3. Department of Surgical Sciences, Anaesthesiology and Intensive Care, Uppsala University, SE-751 85 Uppsala, Sweden

4. Neuroimmunology Unit, Medical School, University of Tampere and Tampere University Hospital, FI-33014 Tampere, Finland

5. Coxa – Hospital for Joint Replacement, FI-33520 Tampere, Finland

6. Department of Anesthesia, Tampere University Hospital, FI-33521 Tampere, Finland

7. Department of Intensive Care Medicine, Kuopio University Hospital, FI-70029 Kuopio, Finland

8. Opthalmology Group, Institute of Biomedical Technology/BioMediTech, University of Tampere, FI-33520 Tampere, Finland

9. The Science Centre of Pirkanmaa Hospital District, FI-33521 Tampere, Finland

Abstract

Summary The possibilities of human pluripotent stem cell-derived neural cells from the basic research tool to a treatment option in regenerative medicine have been well recognized. These cells also offer an interesting tool for in vitro models of neuronal networks to be used for drug screening and neurotoxicological studies and for patient/disease specific in vitro models. Here, as aiming to develop a reductionistic in vitro human neuronal network model, we tested whether human embryonic stem cell (hESC)-derived neural cells could be cultured in human cerebrospinal fluid (CSF) in order to better mimic the in vivo conditions. Our results showed that CSF altered the differentiation of hESC-derived neural cells towards glial cells at the expense of neuronal differentiation. The proliferation rate was reduced in CSF cultures. However, even though the use of CSF as the culture medium altered the glial vs. neuronal differentiation rate, the pre-existing spontaneous activity of the neuronal networks persisted throughout the study. These results suggest that it is possible to develop fully human cell and culture-based environments that can further be modified for various in vitro modeling purposes.

Publisher

The Company of Biologists

Subject

General Agricultural and Biological Sciences,General Biochemistry, Genetics and Molecular Biology

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