Rapid amplification of cDNA end of metallothion in gene during necrosis of plant cells from morinda citrifolia

The objective is to determine the presence of cysteine protease gene in the cDNA fragment being synthesized and determining the efficiency of the 3’RACE PCR approach for amplification of cDNA end. Morinda citrifolia is from the family Rubiaceae. It is the plant with great medicinal values. The prope...

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Main Author: Lee, Jong Jen
Format: Final Year Project Report
Language:English
Published: Universiti Malaysia Sarawak (UNIMAS) 2008
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Online Access:http://ir.unimas.my/id/eprint/7670/3/Lee%20Jong%20Jen.pdf
http://ir.unimas.my/id/eprint/7670/
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Institution: Universiti Malaysia Sarawak
Language: English
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spelling my.unimas.ir.76702023-12-21T07:47:19Z http://ir.unimas.my/id/eprint/7670/ Rapid amplification of cDNA end of metallothion in gene during necrosis of plant cells from morinda citrifolia Lee, Jong Jen SB Plant culture The objective is to determine the presence of cysteine protease gene in the cDNA fragment being synthesized and determining the efficiency of the 3’RACE PCR approach for amplification of cDNA end. Morinda citrifolia is from the family Rubiaceae. It is the plant with great medicinal values. The property of this plant has not been characterized thoroughly in previous time. Cysteine protease play important role in plant growth and development in addition to protein degradation process in plant. Better understanding of the biochemical properties will be attained through the study of cysteine protease gene. The amino acids sequences of this enzyme govern the functional characteristic of this enzyme. Therefore, the termini of the cDNA encoding cysteine protease are amplified through Rapid Amplification of cDNA ends (RACE). This experiment was to amplify the 3’ terminal of the cDNA nucleotide sequence. The RNA extraction was the preliminary step of the reverse transcription reaction to get the coding RNA fragment. First strand cDNA constructed was used for further step of 3’ RACE by using gene specific primer and primers that enabled amplification 3’terminal nucleotides. The PCR products were gel extracted and sent for sequencing. Purified PCR products were cloned for further characterization and analysis of the isolated gene. The gene isolated was found to be similar to metallothionein-like gene and drought stress-induced gene when analysed through Blast. Universiti Malaysia Sarawak (UNIMAS) 2008 Final Year Project Report NonPeerReviewed text en http://ir.unimas.my/id/eprint/7670/3/Lee%20Jong%20Jen.pdf Lee, Jong Jen (2008) Rapid amplification of cDNA end of metallothion in gene during necrosis of plant cells from morinda citrifolia. [Final Year Project Report] (Unpublished)
institution Universiti Malaysia Sarawak
building Centre for Academic Information Services (CAIS)
collection Institutional Repository
continent Asia
country Malaysia
content_provider Universiti Malaysia Sarawak
content_source UNIMAS Institutional Repository
url_provider http://ir.unimas.my/
language English
topic SB Plant culture
spellingShingle SB Plant culture
Lee, Jong Jen
Rapid amplification of cDNA end of metallothion in gene during necrosis of plant cells from morinda citrifolia
description The objective is to determine the presence of cysteine protease gene in the cDNA fragment being synthesized and determining the efficiency of the 3’RACE PCR approach for amplification of cDNA end. Morinda citrifolia is from the family Rubiaceae. It is the plant with great medicinal values. The property of this plant has not been characterized thoroughly in previous time. Cysteine protease play important role in plant growth and development in addition to protein degradation process in plant. Better understanding of the biochemical properties will be attained through the study of cysteine protease gene. The amino acids sequences of this enzyme govern the functional characteristic of this enzyme. Therefore, the termini of the cDNA encoding cysteine protease are amplified through Rapid Amplification of cDNA ends (RACE). This experiment was to amplify the 3’ terminal of the cDNA nucleotide sequence. The RNA extraction was the preliminary step of the reverse transcription reaction to get the coding RNA fragment. First strand cDNA constructed was used for further step of 3’ RACE by using gene specific primer and primers that enabled amplification 3’terminal nucleotides. The PCR products were gel extracted and sent for sequencing. Purified PCR products were cloned for further characterization and analysis of the isolated gene. The gene isolated was found to be similar to metallothionein-like gene and drought stress-induced gene when analysed through Blast.
format Final Year Project Report
author Lee, Jong Jen
author_facet Lee, Jong Jen
author_sort Lee, Jong Jen
title Rapid amplification of cDNA end of metallothion in gene during necrosis of plant cells from morinda citrifolia
title_short Rapid amplification of cDNA end of metallothion in gene during necrosis of plant cells from morinda citrifolia
title_full Rapid amplification of cDNA end of metallothion in gene during necrosis of plant cells from morinda citrifolia
title_fullStr Rapid amplification of cDNA end of metallothion in gene during necrosis of plant cells from morinda citrifolia
title_full_unstemmed Rapid amplification of cDNA end of metallothion in gene during necrosis of plant cells from morinda citrifolia
title_sort rapid amplification of cdna end of metallothion in gene during necrosis of plant cells from morinda citrifolia
publisher Universiti Malaysia Sarawak (UNIMAS)
publishDate 2008
url http://ir.unimas.my/id/eprint/7670/3/Lee%20Jong%20Jen.pdf
http://ir.unimas.my/id/eprint/7670/
_version_ 1787140469922201600