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Production of lentiviral vector with polycistronic transcripts for reprogramming of mouse fibroblast cells

iPS cells were originally generated using monocistronic retroviral vectors carrying the Yamanaka factors 'OSKM'. The development of a polycistronic viral vector with OSKM linked by 2A peptides has simplified reprogramming procedure and reduced the risk of multiple proviral integrations and...

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Main Authors: Al Abbar, Akram, Nordin, Norshariza, Ngai, Siew Ching, Abdullah, Syahrilnizam
Format: Article
Language:English
Published: Universiti Putra Malaysia Press 2018
Online Access:http://psasir.upm.edu.my/id/eprint/66290/1/10%20JST%20Vol%2026%20%282%29%20Apr%202018_JST-0759-2016_pg627-640.pdf
http://psasir.upm.edu.my/id/eprint/66290/
http://www.pertanika.upm.edu.my/Pertanika%20PAPERS/JST%20Vol.%2026%20(2)%20Apr.%202018/10%20JST%20Vol%2026%20(2)%20Apr%202018_JST-0759-2016_pg627-640.pdf
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spelling my.upm.eprints.662902019-02-12T07:01:57Z http://psasir.upm.edu.my/id/eprint/66290/ Production of lentiviral vector with polycistronic transcripts for reprogramming of mouse fibroblast cells Al Abbar, Akram Nordin, Norshariza Ngai, Siew Ching Abdullah, Syahrilnizam iPS cells were originally generated using monocistronic retroviral vectors carrying the Yamanaka factors 'OSKM'. The development of a polycistronic viral vector with OSKM linked by 2A peptides has simplified reprogramming procedure and reduced the risk of multiple proviral integrations and insertional mutagenesis. In this study, we demonstrated the production of the polycistronic lentiviral vector encoding OSKM in a single cassette without a reporter gene or drug-based selection system. Syncytia formations were clearly seen following the co-transfection of a lentiviral plasmid construct with the structural and packaging plasmids. The virion was collected at 48 hours post-transfection. Afterwards, the viral titers were measured by the expression of Sox2 protein from transduced HT1080 cells. Subsequently, Oct4 expression was successfully detected in mouse fibroblasts in the range of 5, 10 and 20 MOIs with expression of 90.7%, 97.5% and 98%, respectively. The results obtained from this study could be used as a model for the production of OSKM lentiviral vector for newcomers to cellular reprogramming research. Universiti Putra Malaysia Press 2018 Article PeerReviewed text en http://psasir.upm.edu.my/id/eprint/66290/1/10%20JST%20Vol%2026%20%282%29%20Apr%202018_JST-0759-2016_pg627-640.pdf Al Abbar, Akram and Nordin, Norshariza and Ngai, Siew Ching and Abdullah, Syahrilnizam (2018) Production of lentiviral vector with polycistronic transcripts for reprogramming of mouse fibroblast cells. Pertanika Journal of Science & Technology, 26 (2). pp. 627-640. ISSN 0128-7680; ESSN: 2231-8526 http://www.pertanika.upm.edu.my/Pertanika%20PAPERS/JST%20Vol.%2026%20(2)%20Apr.%202018/10%20JST%20Vol%2026%20(2)%20Apr%202018_JST-0759-2016_pg627-640.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 iPS cells were originally generated using monocistronic retroviral vectors carrying the Yamanaka factors 'OSKM'. The development of a polycistronic viral vector with OSKM linked by 2A peptides has simplified reprogramming procedure and reduced the risk of multiple proviral integrations and insertional mutagenesis. In this study, we demonstrated the production of the polycistronic lentiviral vector encoding OSKM in a single cassette without a reporter gene or drug-based selection system. Syncytia formations were clearly seen following the co-transfection of a lentiviral plasmid construct with the structural and packaging plasmids. The virion was collected at 48 hours post-transfection. Afterwards, the viral titers were measured by the expression of Sox2 protein from transduced HT1080 cells. Subsequently, Oct4 expression was successfully detected in mouse fibroblasts in the range of 5, 10 and 20 MOIs with expression of 90.7%, 97.5% and 98%, respectively. The results obtained from this study could be used as a model for the production of OSKM lentiviral vector for newcomers to cellular reprogramming research.
format Article
author Al Abbar, Akram
Nordin, Norshariza
Ngai, Siew Ching
Abdullah, Syahrilnizam
spellingShingle Al Abbar, Akram
Nordin, Norshariza
Ngai, Siew Ching
Abdullah, Syahrilnizam
Production of lentiviral vector with polycistronic transcripts for reprogramming of mouse fibroblast cells
author_facet Al Abbar, Akram
Nordin, Norshariza
Ngai, Siew Ching
Abdullah, Syahrilnizam
author_sort Al Abbar, Akram
title Production of lentiviral vector with polycistronic transcripts for reprogramming of mouse fibroblast cells
title_short Production of lentiviral vector with polycistronic transcripts for reprogramming of mouse fibroblast cells
title_full Production of lentiviral vector with polycistronic transcripts for reprogramming of mouse fibroblast cells
title_fullStr Production of lentiviral vector with polycistronic transcripts for reprogramming of mouse fibroblast cells
title_full_unstemmed Production of lentiviral vector with polycistronic transcripts for reprogramming of mouse fibroblast cells
title_sort production of lentiviral vector with polycistronic transcripts for reprogramming of mouse fibroblast cells
publisher Universiti Putra Malaysia Press
publishDate 2018
url http://psasir.upm.edu.my/id/eprint/66290/1/10%20JST%20Vol%2026%20%282%29%20Apr%202018_JST-0759-2016_pg627-640.pdf
http://psasir.upm.edu.my/id/eprint/66290/
http://www.pertanika.upm.edu.my/Pertanika%20PAPERS/JST%20Vol.%2026%20(2)%20Apr.%202018/10%20JST%20Vol%2026%20(2)%20Apr%202018_JST-0759-2016_pg627-640.pdf
_version_ 1643838562602319872
score 13.2014675

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