Protoplast isolation of Boesenbergia Rotunda cell suspension culture / Tan Hao Cheak

Establishment of protoplasts system provides a useful platform for cloning and genetic manipulation of ginger plants. In this study, an efficient protocol for developing protoplast isolation and culture for Boesenbergia rotunda has been established. B. rotunda embryogenic cell suspension cultures sh...

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Main Author: Tan, Hao Cheak
Format: Thesis
Published: 2014
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spelling my.um.stud.47702015-03-04T03:02:15Z Protoplast isolation of Boesenbergia Rotunda cell suspension culture / Tan Hao Cheak Tan, Hao Cheak Q Science (General) QH301 Biology Establishment of protoplasts system provides a useful platform for cloning and genetic manipulation of ginger plants. In this study, an efficient protocol for developing protoplast isolation and culture for Boesenbergia rotunda has been established. B. rotunda embryogenic cell suspension cultures showed good growth rate (μ = 0.1125) when cultured in plant growth regulator (PGR)-free liquid Murashige and Skoog (MS) basal medium supplemented with 3 % sucrose, where no promotive effect were observed in the presence of any concentrations of 2,4-dichlorophenoxyacetic acid (2,4-D) and sonication treatment. This suspension culture was subsequently used as a source to isolate protoplast using enzyme cocktails. A total number of 1 - 5 × 105 per mL protoplasts were isolated using 0.25 % macerozyme and 1 % cellulase incubated for 24 h under continuous shaking condition of 50 rpm in dark condition. Of the isolated protoplasts, 54.93 % were viable according to fluorescein diacetate staining test. About 7.61 ± 1.65 % cultured protoplasts successfully formed micro-colonies when cultured in liquid MS basal medium supplemented with 9 g/L mannitol, 2 mg/L 1-naphthaleacetic acid (NAA), 0.5 mg/L benzylaminopurine (BAP) and incubated at 25 ± 2 °C in dark condition for 4 weeks. The osmoticum of the culture media were reduced weekly during the protoplast culture period from 9 to 5 % followed by 1 %. These colonies were subsequently transferred to solid MS medium supplemented with 0.5 mg/L BAP for callus initiation. The callus was formed after 5 weeks of culture. 2014 Thesis NonPeerReviewed application/pdf http://studentsrepo.um.edu.my/4770/1/0COVER_%2D_(TAN_HAO_CHEAK%2D_SGF_%2D_ISB).pdf application/pdf http://studentsrepo.um.edu.my/4770/2/1COVER_%2D_(TAN_HAO_CHEAK%2D_SGF_%2D_ISB).pdf application/pdf http://studentsrepo.um.edu.my/4770/3/2Form%2D_Original_Literary_Work_Declaration.pdf application/pdf http://studentsrepo.um.edu.my/4770/4/3Thesis_2.pdf application/pdf http://studentsrepo.um.edu.my/4770/5/4Thesis_3.pdf Tan, Hao Cheak (2014) Protoplast isolation of Boesenbergia Rotunda cell suspension culture / Tan Hao Cheak. Masters thesis, University of Malaya. http://studentsrepo.um.edu.my/4770/
institution Universiti Malaya
building UM Library
collection Institutional Repository
continent Asia
country Malaysia
content_provider Universiti Malaya
content_source UM Student Repository
url_provider http://studentsrepo.um.edu.my/
topic Q Science (General)
QH301 Biology
spellingShingle Q Science (General)
QH301 Biology
Tan, Hao Cheak
Protoplast isolation of Boesenbergia Rotunda cell suspension culture / Tan Hao Cheak
description Establishment of protoplasts system provides a useful platform for cloning and genetic manipulation of ginger plants. In this study, an efficient protocol for developing protoplast isolation and culture for Boesenbergia rotunda has been established. B. rotunda embryogenic cell suspension cultures showed good growth rate (μ = 0.1125) when cultured in plant growth regulator (PGR)-free liquid Murashige and Skoog (MS) basal medium supplemented with 3 % sucrose, where no promotive effect were observed in the presence of any concentrations of 2,4-dichlorophenoxyacetic acid (2,4-D) and sonication treatment. This suspension culture was subsequently used as a source to isolate protoplast using enzyme cocktails. A total number of 1 - 5 × 105 per mL protoplasts were isolated using 0.25 % macerozyme and 1 % cellulase incubated for 24 h under continuous shaking condition of 50 rpm in dark condition. Of the isolated protoplasts, 54.93 % were viable according to fluorescein diacetate staining test. About 7.61 ± 1.65 % cultured protoplasts successfully formed micro-colonies when cultured in liquid MS basal medium supplemented with 9 g/L mannitol, 2 mg/L 1-naphthaleacetic acid (NAA), 0.5 mg/L benzylaminopurine (BAP) and incubated at 25 ± 2 °C in dark condition for 4 weeks. The osmoticum of the culture media were reduced weekly during the protoplast culture period from 9 to 5 % followed by 1 %. These colonies were subsequently transferred to solid MS medium supplemented with 0.5 mg/L BAP for callus initiation. The callus was formed after 5 weeks of culture.
format Thesis
author Tan, Hao Cheak
author_facet Tan, Hao Cheak
author_sort Tan, Hao Cheak
title Protoplast isolation of Boesenbergia Rotunda cell suspension culture / Tan Hao Cheak
title_short Protoplast isolation of Boesenbergia Rotunda cell suspension culture / Tan Hao Cheak
title_full Protoplast isolation of Boesenbergia Rotunda cell suspension culture / Tan Hao Cheak
title_fullStr Protoplast isolation of Boesenbergia Rotunda cell suspension culture / Tan Hao Cheak
title_full_unstemmed Protoplast isolation of Boesenbergia Rotunda cell suspension culture / Tan Hao Cheak
title_sort protoplast isolation of boesenbergia rotunda cell suspension culture / tan hao cheak
publishDate 2014
url http://studentsrepo.um.edu.my/4770/1/0COVER_%2D_(TAN_HAO_CHEAK%2D_SGF_%2D_ISB).pdf
http://studentsrepo.um.edu.my/4770/2/1COVER_%2D_(TAN_HAO_CHEAK%2D_SGF_%2D_ISB).pdf
http://studentsrepo.um.edu.my/4770/3/2Form%2D_Original_Literary_Work_Declaration.pdf
http://studentsrepo.um.edu.my/4770/4/3Thesis_2.pdf
http://studentsrepo.um.edu.my/4770/5/4Thesis_3.pdf
http://studentsrepo.um.edu.my/4770/
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