Quantification of infectious recombinant murine MSCV-based retroviruses using PCR approach

The current available molecular method to detect the retroviral-mediated gene expression is reverse transcriptase-polymerase chain reaction (RT-PCR). However, the conventional PCR is time consuming, prone to error and not sensitive. In this paper, we performed a real-time PCR assay to quantify retro...

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Main Authors: Nik Abd Rahman, Nik Mohd Afizan, Allaudin, Zeenathul Nazariah, Ismail, Ruzila, Mustafa, Nor Hidayah, Mohd Lila, Mohd Azmi
Format: Article
Language:English
Published: EuroJournals Publishing 2010
Online Access:http://psasir.upm.edu.my/id/eprint/16410/1/Quantification%20of%20infectious%20recombinant%20murine%20MSCV.pdf
http://psasir.upm.edu.my/id/eprint/16410/
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Institution: Universiti Putra Malaysia
Language: English
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spelling my.upm.eprints.164102019-10-30T06:16:50Z http://psasir.upm.edu.my/id/eprint/16410/ Quantification of infectious recombinant murine MSCV-based retroviruses using PCR approach Nik Abd Rahman, Nik Mohd Afizan Allaudin, Zeenathul Nazariah Ismail, Ruzila Mustafa, Nor Hidayah Mohd Lila, Mohd Azmi The current available molecular method to detect the retroviral-mediated gene expression is reverse transcriptase-polymerase chain reaction (RT-PCR). However, the conventional PCR is time consuming, prone to error and not sensitive. In this paper, we performed a real-time PCR assay to quantify retroviral mediated gene expression in the supernatant of infectious recombinant virus. We documented an optimized methodology for accurate and reproducible quantification of retrovirus-based gene expression which enables rapid and quantitative determination of sample gene expression. We have also compared the performance of the assay with our routine RT-PCR assay. RNA was extracted from infectious recombinant retrovirus at 48 h post-infection and assayed for VP3 gene. The standard curve from linear DNA standards showed high sensitivity and good linearity (R2 = 0.9902 for VP3 standards graphs), ranged from 102 to 108 copies of comparable accuracy to current quantification real-time PCR methods. The present study presumes a copy number of transgene expression to equal a molecule of infectious recombinant virus particle. Another advantage, this concept could determine vector stability by comparison of infectious particles, total particles and particles with RNA. In comparison to gel-based RTPCR, we conclude that real-time PCR as a better approach in gene expression quantification. EuroJournals Publishing 2010-09-16 Article PeerReviewed application/pdf en http://psasir.upm.edu.my/id/eprint/16410/1/Quantification%20of%20infectious%20recombinant%20murine%20MSCV.pdf Nik Abd Rahman, Nik Mohd Afizan and Allaudin, Zeenathul Nazariah and Ismail, Ruzila and Mustafa, Nor Hidayah and Mohd Lila, Mohd Azmi (2010) Quantification of infectious recombinant murine MSCV-based retroviruses using PCR approach. Research Journal of International Studies, 16. pp. 5-14. ISSN 1453-212X
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 The current available molecular method to detect the retroviral-mediated gene expression is reverse transcriptase-polymerase chain reaction (RT-PCR). However, the conventional PCR is time consuming, prone to error and not sensitive. In this paper, we performed a real-time PCR assay to quantify retroviral mediated gene expression in the supernatant of infectious recombinant virus. We documented an optimized methodology for accurate and reproducible quantification of retrovirus-based gene expression which enables rapid and quantitative determination of sample gene expression. We have also compared the performance of the assay with our routine RT-PCR assay. RNA was extracted from infectious recombinant retrovirus at 48 h post-infection and assayed for VP3 gene. The standard curve from linear DNA standards showed high sensitivity and good linearity (R2 = 0.9902 for VP3 standards graphs), ranged from 102 to 108 copies of comparable accuracy to current quantification real-time PCR methods. The present study presumes a copy number of transgene expression to equal a molecule of infectious recombinant virus particle. Another advantage, this concept could determine vector stability by comparison of infectious particles, total particles and particles with RNA. In comparison to gel-based RTPCR, we conclude that real-time PCR as a better approach in gene expression quantification.
format Article
author Nik Abd Rahman, Nik Mohd Afizan
Allaudin, Zeenathul Nazariah
Ismail, Ruzila
Mustafa, Nor Hidayah
Mohd Lila, Mohd Azmi
spellingShingle Nik Abd Rahman, Nik Mohd Afizan
Allaudin, Zeenathul Nazariah
Ismail, Ruzila
Mustafa, Nor Hidayah
Mohd Lila, Mohd Azmi
Quantification of infectious recombinant murine MSCV-based retroviruses using PCR approach
author_facet Nik Abd Rahman, Nik Mohd Afizan
Allaudin, Zeenathul Nazariah
Ismail, Ruzila
Mustafa, Nor Hidayah
Mohd Lila, Mohd Azmi
author_sort Nik Abd Rahman, Nik Mohd Afizan
title Quantification of infectious recombinant murine MSCV-based retroviruses using PCR approach
title_short Quantification of infectious recombinant murine MSCV-based retroviruses using PCR approach
title_full Quantification of infectious recombinant murine MSCV-based retroviruses using PCR approach
title_fullStr Quantification of infectious recombinant murine MSCV-based retroviruses using PCR approach
title_full_unstemmed Quantification of infectious recombinant murine MSCV-based retroviruses using PCR approach
title_sort quantification of infectious recombinant murine mscv-based retroviruses using pcr approach
publisher EuroJournals Publishing
publishDate 2010
url http://psasir.upm.edu.my/id/eprint/16410/1/Quantification%20of%20infectious%20recombinant%20murine%20MSCV.pdf
http://psasir.upm.edu.my/id/eprint/16410/
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