A Simplified Method For Isolation and Culture of Neural Stem Cells From Adult Mice Brain: in Vitro

The present study aimed to develop an uncomplicated method for isolation and culture of mice brain derived-neural stem cells (NSCs) - neurospheres, using a simplified method. In order to obtain single cells suspension, the brain tissue was dissociated using mechanical methods (trituration) instead o...

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Main Authors: Nashaat G. Mustafa, Intissar N. Waheed, Sa'ad G. Salih
Format: Article
Language:English
Published: University of Zakho 2013-09-01
Series:Science Journal of University of Zakho
Subjects:
Online Access:https://sjuoz.uoz.edu.krd/index.php/sjuoz/article/view/261
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spelling doaj-315e26fff8844dd7acb61474f4474d452020-11-25T00:44:51Zeng University of ZakhoScience Journal of University of Zakho2663-628X2663-62982013-09-0112525532261A Simplified Method For Isolation and Culture of Neural Stem Cells From Adult Mice Brain: in VitroNashaat G. Mustafa0Intissar N. Waheed1Sa'ad G. Salih2University of MosulUniversity of ZakhoUniversity of MosulThe present study aimed to develop an uncomplicated method for isolation and culture of mice brain derived-neural stem cells (NSCs) - neurospheres, using a simplified method. In order to obtain single cells suspension, the brain tissue was dissociated using mechanical methods (trituration) instead of enzymatic method. These single cells suspension were in vitro cultured in DMEM)/Ham's F12 (1:1) mixture (high glucose) plus 20 ng/ml Epidermal growth factor (rHuEGF) and 20 ng/ml Fibroblast growth factor-basic (FGF-2). The results showed the combined actions of rHuEGF and bFGF-2 was in inducing proliferation of brain derived-NSCs. So, after 3 days culture numerous number of NSCs were observed floated in culture medium. Then within the time of culture the numbers of NSCs were increased. After 7 days culture some of these cells began to aggregate and form small sized neurosphere of undifferentiated cells (early stage) and within 3 weeks culture, large sized mature neurospheres were formed. When these neurospheres were aspirated and re-cultured on the gelatin pre- coated Petri dish, these neurospheres were attached and several nerve cells began to migrate from these neurospheres and occupy the surrounding area. This result confirms the incidence of NSCs derived neurospheres and it is ability to differentiate to nerve cell.  In conclusion this method is simple and less expensive, less effort, but take longer time to get NSCs derived-neurosphere, as well as it is possible to use mechanical dissociation of cells (trituration) instead of enzymatic method to obtain single cell suspension.https://sjuoz.uoz.edu.krd/index.php/sjuoz/article/view/261Neural stem cellsNeurosphereMice brainin vitro
collection DOAJ
language English
format Article
sources DOAJ
author Nashaat G. Mustafa
Intissar N. Waheed
Sa'ad G. Salih
spellingShingle Nashaat G. Mustafa
Intissar N. Waheed
Sa'ad G. Salih
A Simplified Method For Isolation and Culture of Neural Stem Cells From Adult Mice Brain: in Vitro
Science Journal of University of Zakho
Neural stem cells
Neurosphere
Mice brain
in vitro
author_facet Nashaat G. Mustafa
Intissar N. Waheed
Sa'ad G. Salih
author_sort Nashaat G. Mustafa
title A Simplified Method For Isolation and Culture of Neural Stem Cells From Adult Mice Brain: in Vitro
title_short A Simplified Method For Isolation and Culture of Neural Stem Cells From Adult Mice Brain: in Vitro
title_full A Simplified Method For Isolation and Culture of Neural Stem Cells From Adult Mice Brain: in Vitro
title_fullStr A Simplified Method For Isolation and Culture of Neural Stem Cells From Adult Mice Brain: in Vitro
title_full_unstemmed A Simplified Method For Isolation and Culture of Neural Stem Cells From Adult Mice Brain: in Vitro
title_sort simplified method for isolation and culture of neural stem cells from adult mice brain: in vitro
publisher University of Zakho
series Science Journal of University of Zakho
issn 2663-628X
2663-6298
publishDate 2013-09-01
description The present study aimed to develop an uncomplicated method for isolation and culture of mice brain derived-neural stem cells (NSCs) - neurospheres, using a simplified method. In order to obtain single cells suspension, the brain tissue was dissociated using mechanical methods (trituration) instead of enzymatic method. These single cells suspension were in vitro cultured in DMEM)/Ham's F12 (1:1) mixture (high glucose) plus 20 ng/ml Epidermal growth factor (rHuEGF) and 20 ng/ml Fibroblast growth factor-basic (FGF-2). The results showed the combined actions of rHuEGF and bFGF-2 was in inducing proliferation of brain derived-NSCs. So, after 3 days culture numerous number of NSCs were observed floated in culture medium. Then within the time of culture the numbers of NSCs were increased. After 7 days culture some of these cells began to aggregate and form small sized neurosphere of undifferentiated cells (early stage) and within 3 weeks culture, large sized mature neurospheres were formed. When these neurospheres were aspirated and re-cultured on the gelatin pre- coated Petri dish, these neurospheres were attached and several nerve cells began to migrate from these neurospheres and occupy the surrounding area. This result confirms the incidence of NSCs derived neurospheres and it is ability to differentiate to nerve cell.  In conclusion this method is simple and less expensive, less effort, but take longer time to get NSCs derived-neurosphere, as well as it is possible to use mechanical dissociation of cells (trituration) instead of enzymatic method to obtain single cell suspension.
topic Neural stem cells
Neurosphere
Mice brain
in vitro
url https://sjuoz.uoz.edu.krd/index.php/sjuoz/article/view/261
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