Evaluation of two cell culture media in culturing rat full term amniotic fluid cells

Introduction: Amniotic fluid (AF) consists of heterogenous population of cells with high diagnostic and therapeutic values. The study of rat amniotic fluid cells is very limited, despite the extensive use of this animal model in biomedical research. Primary culture of rat AF cells, especially from f...

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Main Authors: Ferdaos, Nurfarhana, Karrupiah, Thilakavathy, Rosli, Rozita, Yazid, Mohd Nazri, Nordin, Norshariza
Format: Article
Language:English
Published: Faculty of Medicine and Health Sciences, Universiti Putra Malaysia 2011
Online Access:http://psasir.upm.edu.my/id/eprint/24610/1/Evaluation%20of%20Two%20Cell%20Culture%20Media%20in%20Culturing%20Rat%20Full%20Term.pdf
http://psasir.upm.edu.my/id/eprint/24610/
http://www.medic.upm.edu.my/dokumen/FKUSK1_MJMHS_2011V07N2_OP09.pdf
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spelling my.upm.eprints.246102015-09-08T02:44:15Z http://psasir.upm.edu.my/id/eprint/24610/ Evaluation of two cell culture media in culturing rat full term amniotic fluid cells Ferdaos, Nurfarhana Karrupiah, Thilakavathy Rosli, Rozita Yazid, Mohd Nazri Nordin, Norshariza Introduction: Amniotic fluid (AF) consists of heterogenous population of cells with high diagnostic and therapeutic values. The study of rat amniotic fluid cells is very limited, despite the extensive use of this animal model in biomedical research. Primary culture of rat AF cells, especially from full term pregnancies has not been well established. Here we attempt to determine the suitable medium in culturing rat AF cells that would enhance the cell viability, growth rate and heterogeneity. Methods: The cell viability, growth rate and heterogeneity of rat AF cells were compared upon culturing the primary cells in two different media; Amniomax or RPMI. Cell viability study was carried out using trypan blue staining, while the growth rate was monitored based on the time required to passage the cells (population doubling time in hour). The heterogeneity of cells was examined based on the morphology of the cells. Statistical analysis was performed using t-test. Results: Amniomax was observed to provide a better culture condition in culturing rat AF cells as the cells are more viable, grow faster and more heterogenous as compared to the cells grown in RPMI. Conclusion: Amniomax is a more suitable medium for high quality and viability of full term rat AF cell culture, as compared to RPMI. Thus, warranting propagation of more rat AF cells for biomedical research. Faculty of Medicine and Health Sciences, Universiti Putra Malaysia 2011-06 Article PeerReviewed application/pdf en http://psasir.upm.edu.my/id/eprint/24610/1/Evaluation%20of%20Two%20Cell%20Culture%20Media%20in%20Culturing%20Rat%20Full%20Term.pdf Ferdaos, Nurfarhana and Karrupiah, Thilakavathy and Rosli, Rozita and Yazid, Mohd Nazri and Nordin, Norshariza (2011) Evaluation of two cell culture media in culturing rat full term amniotic fluid cells. Malaysian Journal of Medicine and Health Sciences, 7 (2). pp. 81-85. ISSN 1675-8544 http://www.medic.upm.edu.my/dokumen/FKUSK1_MJMHS_2011V07N2_OP09.pdf
institution Universiti Putra Malaysia
building UPM Library
collection Institutional Repository
continent Asia
country Malaysia
content_provider Universiti Putra Malaysia
content_source UPM Institutional Repository
url_provider http://psasir.upm.edu.my/
language English
description Introduction: Amniotic fluid (AF) consists of heterogenous population of cells with high diagnostic and therapeutic values. The study of rat amniotic fluid cells is very limited, despite the extensive use of this animal model in biomedical research. Primary culture of rat AF cells, especially from full term pregnancies has not been well established. Here we attempt to determine the suitable medium in culturing rat AF cells that would enhance the cell viability, growth rate and heterogeneity. Methods: The cell viability, growth rate and heterogeneity of rat AF cells were compared upon culturing the primary cells in two different media; Amniomax or RPMI. Cell viability study was carried out using trypan blue staining, while the growth rate was monitored based on the time required to passage the cells (population doubling time in hour). The heterogeneity of cells was examined based on the morphology of the cells. Statistical analysis was performed using t-test. Results: Amniomax was observed to provide a better culture condition in culturing rat AF cells as the cells are more viable, grow faster and more heterogenous as compared to the cells grown in RPMI. Conclusion: Amniomax is a more suitable medium for high quality and viability of full term rat AF cell culture, as compared to RPMI. Thus, warranting propagation of more rat AF cells for biomedical research.
format Article
author Ferdaos, Nurfarhana
Karrupiah, Thilakavathy
Rosli, Rozita
Yazid, Mohd Nazri
Nordin, Norshariza
spellingShingle Ferdaos, Nurfarhana
Karrupiah, Thilakavathy
Rosli, Rozita
Yazid, Mohd Nazri
Nordin, Norshariza
Evaluation of two cell culture media in culturing rat full term amniotic fluid cells
author_facet Ferdaos, Nurfarhana
Karrupiah, Thilakavathy
Rosli, Rozita
Yazid, Mohd Nazri
Nordin, Norshariza
author_sort Ferdaos, Nurfarhana
title Evaluation of two cell culture media in culturing rat full term amniotic fluid cells
title_short Evaluation of two cell culture media in culturing rat full term amniotic fluid cells
title_full Evaluation of two cell culture media in culturing rat full term amniotic fluid cells
title_fullStr Evaluation of two cell culture media in culturing rat full term amniotic fluid cells
title_full_unstemmed Evaluation of two cell culture media in culturing rat full term amniotic fluid cells
title_sort evaluation of two cell culture media in culturing rat full term amniotic fluid cells
publisher Faculty of Medicine and Health Sciences, Universiti Putra Malaysia
publishDate 2011
url http://psasir.upm.edu.my/id/eprint/24610/1/Evaluation%20of%20Two%20Cell%20Culture%20Media%20in%20Culturing%20Rat%20Full%20Term.pdf
http://psasir.upm.edu.my/id/eprint/24610/
http://www.medic.upm.edu.my/dokumen/FKUSK1_MJMHS_2011V07N2_OP09.pdf
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