IIUM Repository

Gene expression of Anx3 in Pb-treated Nicotiana tabacum using a real-time RT-PCR

Phang, Ing Chia and Nawi, Mohd Afiq and Razak, Nurhayati and Ismail, Nor Adibah and Pappusamy, Arokiaraj (2012) Gene expression of Anx3 in Pb-treated Nicotiana tabacum using a real-time RT-PCR. In: 15th International Biotechnology Symposium (IBS) and Exhibition, IBS 2012: Innovative Biotechnology for a Green World and Beyond, 16 - 21 September 2012, Daegu, South Korea.

[img] PDF - Published Version
Restricted to Repository staff only

Download (1MB) | Request a copy
[img]
Preview
PDF (Gene expression of Anx3 in Pb-treated Nicotiana tabacum using a real-time RT-PCR) - Cover Image
Download (233kB) | Preview
Official URL: http://www.ibs2012.org/

Abstract

Lead (Pb) is one of the highly persistent, toxic, and widely distributed heavy metal pollutants in the environment. This heavy metal has a tendency to enter human food chain, thus affecting public health. One effective way to remove heavy metals pollutant is by using plants, a technology known as phytoremediation. One such plant that is routinely employed as an experimental model for such studies is Nicotiana tabacum. As tobacco plants are not generally consumed by herbivores, it minimizes the possibility of Pb from entering food chain. A number of studies suggest that annexins, a calcium-binding protein, does play a role in plant stress response. The expression of annexin gene in plants appeared to be regulated by tissue-specific developmental and environmental signal. A vacuole-associated annexin from N. tabacum, Anx3, was investigated, to observe the involvement of this gene in Pb-induced stress. Reverse transcription following quantitative real-time 0olymerase chain reaction (qRT-PCR) is a useful analysis to study gene expression. In this analysis, a reference gene that acts as internal control (housekeeping gene) is routinely employed for normalization of qRT-PCR against the target gene (Anx3). The candidate reference genes, L25, EF-1α, and Ntubc2, were evaluated using suitable primer pairs in order to select the most stable reference gene for normalization of qRT-PCR in this study. Using geNorm, NormFinder, and BestKeeper programs, the most suitable reference gene identified in this study was L25. The relative quantification of Anx3 gene expression normalizing against L25 was accomplished by REST software. The expression level of Anx3 in Pb-treated N. tabacum was upregulated by 2.2-fold (p < 0.05). The experimental methods used and the participation of Anx3 in defense against Pb stress will be discussed.

Item Type: Conference or Workshop Item (Poster)
Additional Information: 6480/26412
Uncontrolled Keywords: Lead (Pb), Anx3, Nicotiana tabacum, real-time RT-PCR, reference gene
Subjects: Q Science > Q Science (General)
Kulliyyahs/Centres/Divisions/Institutes (Can select more than one option. Press CONTROL button): Kulliyyah of Science > Department of Biotechnology
Depositing User: Dr. Ing Chia Phang
Date Deposited: 18 Dec 2012 14:51
Last Modified: 18 Dec 2012 14:51
URI: http://irep.iium.edu.my/id/eprint/26412

Actions (login required)

View Item View Item

Downloads

Downloads per month over past year