Hevea genetic transformation for enhanced recombinant pharmaceutical production by the use of hevein promoter

Pharmaceuticals produced in the latex cytosol of genetically transformed Hevea can be harvested nondestructively by conventional tapping. This study evaluates the promoter activity of the 5’-untranslated upstream regulating region of hevein gene, which encodes the most abundant soluble protein in H...

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Main Authors: Pappusamy, Arokiaraj, Shuib, Siti Shuhada, Badaruddin, Badrul Ezam, Sunderasan, E.
Format: Conference or Workshop Item
Language:English
Published: 2010
Subjects:
Online Access:http://irep.iium.edu.my/15900/1/2010_IRIIE_Kamarul_et_al_Aromatic.pdf
http://irep.iium.edu.my/15900/
http://www.iium.edu.my/irie/10/info/Programme_Book%20Part_2.pdf
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Institution: Universiti Islam Antarabangsa Malaysia
Language: English
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spelling my.iium.irep.159002012-01-30T00:06:48Z http://irep.iium.edu.my/15900/ Hevea genetic transformation for enhanced recombinant pharmaceutical production by the use of hevein promoter Pappusamy, Arokiaraj Shuib, Siti Shuhada Badaruddin, Badrul Ezam Sunderasan, E. TP248.13 Biotechnology Pharmaceuticals produced in the latex cytosol of genetically transformed Hevea can be harvested nondestructively by conventional tapping. This study evaluates the promoter activity of the 5’-untranslated upstream regulating region of hevein gene, which encodes the most abundant soluble protein in Hevea latex. Constructs were prepared with the test hevein promoter fragments Hev P1 (0.35kb), Hev P2 (0.45kb) and Hev P3 (0.73kb) that were inserted 5’ to the pharmaceutical genes i.e. human protamine 1 (HP1) and human atrial natriur tic factor (HANF), in pGPTV-Kan expression vector. The expression vectors containing HP1 and HANF were electroporated into Agrobacterium tumefaciens GV2260 containing supervirulent plasmid pToK47, which were then used to infect Hevea anther callus. The growth of the putative transformed Hevea callus was monitored on kanamycin selection media. The presence of the pharmaceutical genes (HP1 and HANF), the hevein promoter fragments, and nptII selection marker were verified by PCR on sampled putative transformed callus. The remaining callus tissues will be sub-cultured and transferred into differentiation media for embryoids formation and plantlet regeneration. 2010 Conference or Workshop Item REM application/pdf en http://irep.iium.edu.my/15900/1/2010_IRIIE_Kamarul_et_al_Aromatic.pdf Pappusamy, Arokiaraj and Shuib, Siti Shuhada and Badaruddin, Badrul Ezam and Sunderasan, E. (2010) Hevea genetic transformation for enhanced recombinant pharmaceutical production by the use of hevein promoter. In: IIUM Research, Innovation & Invention Exhibition (IRIIE 2010), 26 - 27 January 2010, Kuala Lumpur. http://www.iium.edu.my/irie/10/info/Programme_Book%20Part_2.pdf
institution Universiti Islam Antarabangsa Malaysia
building IIUM Library
collection Institutional Repository
continent Asia
country Malaysia
content_provider International Islamic University Malaysia
content_source IIUM Repository (IREP)
url_provider http://irep.iium.edu.my/
language English
topic TP248.13 Biotechnology
spellingShingle TP248.13 Biotechnology
Pappusamy, Arokiaraj
Shuib, Siti Shuhada
Badaruddin, Badrul Ezam
Sunderasan, E.
Hevea genetic transformation for enhanced recombinant pharmaceutical production by the use of hevein promoter
description Pharmaceuticals produced in the latex cytosol of genetically transformed Hevea can be harvested nondestructively by conventional tapping. This study evaluates the promoter activity of the 5’-untranslated upstream regulating region of hevein gene, which encodes the most abundant soluble protein in Hevea latex. Constructs were prepared with the test hevein promoter fragments Hev P1 (0.35kb), Hev P2 (0.45kb) and Hev P3 (0.73kb) that were inserted 5’ to the pharmaceutical genes i.e. human protamine 1 (HP1) and human atrial natriur tic factor (HANF), in pGPTV-Kan expression vector. The expression vectors containing HP1 and HANF were electroporated into Agrobacterium tumefaciens GV2260 containing supervirulent plasmid pToK47, which were then used to infect Hevea anther callus. The growth of the putative transformed Hevea callus was monitored on kanamycin selection media. The presence of the pharmaceutical genes (HP1 and HANF), the hevein promoter fragments, and nptII selection marker were verified by PCR on sampled putative transformed callus. The remaining callus tissues will be sub-cultured and transferred into differentiation media for embryoids formation and plantlet regeneration.
format Conference or Workshop Item
author Pappusamy, Arokiaraj
Shuib, Siti Shuhada
Badaruddin, Badrul Ezam
Sunderasan, E.
author_facet Pappusamy, Arokiaraj
Shuib, Siti Shuhada
Badaruddin, Badrul Ezam
Sunderasan, E.
author_sort Pappusamy, Arokiaraj
title Hevea genetic transformation for enhanced recombinant pharmaceutical production by the use of hevein promoter
title_short Hevea genetic transformation for enhanced recombinant pharmaceutical production by the use of hevein promoter
title_full Hevea genetic transformation for enhanced recombinant pharmaceutical production by the use of hevein promoter
title_fullStr Hevea genetic transformation for enhanced recombinant pharmaceutical production by the use of hevein promoter
title_full_unstemmed Hevea genetic transformation for enhanced recombinant pharmaceutical production by the use of hevein promoter
title_sort hevea genetic transformation for enhanced recombinant pharmaceutical production by the use of hevein promoter
publishDate 2010
url http://irep.iium.edu.my/15900/1/2010_IRIIE_Kamarul_et_al_Aromatic.pdf
http://irep.iium.edu.my/15900/
http://www.iium.edu.my/irie/10/info/Programme_Book%20Part_2.pdf
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