Purpose:To study preliminarily in vitro induced differentiation of embryonic stem cells into neurons for further investigation of an alternative for the treatment of glaumatous neuropathy.Materials and methods:Supernatant of cultured Buffalo rat liver cells(buffalorat liver cell-conditioned medium,BRL-CM)was used for culturing embryonic stem cells(ES-D3 cell line),Morphological features of undifferentiated EScells were studied by HE staining and electron microscopy.Based on the methods used by Bain et al,we modified the methods and used retinoic acid(RA)as an inducer to differentiate ES-D3 cells and cytosine arabinoside(Ara-C)as inhibitor of proliferative cells.The growth of the cells was observed under phase contrast microscope.Results:ES-D3cells cultured by BRL-CMgrew in aggregates and remained undifferentiated.Electromicroscopy showed large nucleus and a large amount of mitochondria in undifferentiated ES cells and many processes on the surfaces.In the first day after the adding of retinoic acid,some neuron-like cells with one,two or more processes were present.In the second day after adding RAand the first day after the plus of 10μm Ara-C,a large amount of neuron-like cells appeared,with the formation of neuron-like networks.Con clusions:Combined use of RA and Ara-Ccan induce ES cells to differentiate into neuron-like cells.Our present preliminary study might provide insights into an alternative for the treatment of glaucomatous neuropathy by the transplantation of embryonic stem cells.Eye Science2000;16:1-6.
Purpose:To investigate the influencing factors in culturing Srague-Dawley(S-D) rats retinal neurons in order to lay foundation for further experimental research.Materials and Methods:Retinal cells were plated on plastic plates and coverslips coated with poly-lysine or ethylene imine polymer for primary culture.The cultured cells were divided into following groups:1.Culture medium changed every 2 tp 3 days vs changed only once;2.Cytosine arabinoside(Ara-C)added to the culture medium vs not added.The cells were observed and pictured under inverted phase contrast microscope.The cells were identified through immunocytochemistry.Results:The immunofluorescence showed that most of the cultured cells were neurons,among them were a few retinal ganglion cells.In the cultured group of which substrata coated with poly-l-lysine and culture medium added with Ara-c,the neurons intended to aggregate into clusters with relatively straight neurites.In the group of which substrata coated with ethylene imine polymer and medium added with Ara-c,the neurons grew dispersively with bent neurites.Both of them survived for 2 to 3 weeks.The cells which plated in the medium not added with Ara-c did not aggregate into clusters and survived longer than 4 weeks.In the group of which medium changed several times,the survival time of neurons was shorter than that in the medium changed only once.Conclusions:The retinal neurons plated on the substrata coated with ethylene imine polymer are easy to observe because of its dispersive growth.It is not favorable for the growth of the neurons by changing culture medium many times.Ara-c may possibly have side effect on the growth of retinal neurons.
