Schwann cell cultures from human fetal dorsal root ganglia

来源 :Neural Regeneration Research | 被引量 : 0次 | 上传用户:wdelaopologo
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BACKGROUND:Previous studies have used many methods for in vitro Schwann cells(SCs) cultures and purification,such as single cell suspension and cytosine arabinoside.However,it has been difficult to obtain sufficient cellular density,and the procedures have been quite tedious. OBJECTIVE:To investigate the feasibility of culturing high-density SCs using fetal human dorsal root ganglion tissue explants. DESIGN,TIME AND SETTING:Cell culture and immunohistochemistry were performed at the Central Laboratory of Kunming General Hospital of Chinese PLA between March 2001 and October 2008. MATERIALS:Culture media containing 10%fetal bovine serum,as well as 0.2%collagenase and 0.25%trypsin were purchased from Gibco,USA;mouse anti-human S-100 monoclonal antibody and goat anti-mouse IgG labeled with horseradish peroxidase were provided by Beijing Institute of Biological Products,China. METHODS:Primarily cultured SCs were dissociated from dorsal root ganglia of human aborted fetuses at 4-6 months pregnancy.Following removal of the dorsal root ganglion perineurium,the ganglia were dissected into tiny pieces and digested with 0.2%collagenase and 0.25%trypsin (volume ratio 1:1),then explanted and cultured.SC purification was performed with 5 mL 10%fetal bovine serum added to the culture media,followed by differential adhesion. MAIN OUTCOME MEASURES:SCs morphology was observed under inverted phase contrast light microscopy.SC purity was evaluated according to percentage of S-100 immunostained cells. RESULTS:SCs were primarily cultured for 5 6 days and then subcultured for 4 5 passages.The highly enriched SC population reached>95%purity and presented with normal morphology. CONCLUSION:A high purity of SCs was obtained with culture methods using human fetal dorsal root qanqlion tissue explants. BACKGROUND: Previous studies have used many methods for in vitro cultures and purifications, such as single cell suspension and cytosine arabinoside. It has been difficult to obtain sufficient cellular density, and the procedures have been quite tedious. OBJECTIVE : To investigate the feasibility of culturing high-density SCs using fetal human dorsal root ganglion tissue explants. DESIGN, TIME AND SETTING: Cell culture and immunohistochemistry were performed at the Central Laboratory of Kunming General Hospital of Chinese PLA between March 2001 and October 2008. MATERIALS: Culture medium containing 10% fetal bovine serum, as well as 0.2% collagenase and 0.25% trypsin were purchased from Gibco, USA; mouse anti-human S-100 monoclonal antibody and goat anti-mouse IgG labeled with horseradish peroxidase were provided by Beijing Institute of Biological Products, China. METHODS: Primarily cultured SCs were dissociated from dorsal root ganglia of human aborted fetuses at 4-6 months pr egnancy. Cooling removed of the dorsal root ganglion perineurium, the ganglia were dissected into tiny pieces and digested with 0.2% collagenase and 0.25% trypsin (volume ratio 1: 1), then explanted and cultured. SC purification was performed with 5 mL of 10% fetal bovine serum added to the culture media, followed by differential adhesion. MAIN OUTCOME MEASURES: SCs morphology was observed under inverted phase contrast light microscopy. SC purity was evaluated according to percentage of S-100 immunostained cells. CONCLUSION: A high purity of SCs was obtained with culture methods using human fetal dorsal root qanqlion tissue explants.
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