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  1. NTU Theses and Dissertations Repository
  2. 生物資源暨農學院
  3. 森林環境暨資源學系
請用此 Handle URI 來引用此文件: http://tdr.lib.ntu.edu.tw/jspui/handle/123456789/62529
完整後設資料紀錄
DC 欄位值語言
dc.contributor.advisor王亞男
dc.contributor.authorChien-Chen Huangen
dc.contributor.author黃千真zh_TW
dc.date.accessioned2021-06-16T16:03:53Z-
dc.date.available2013-09-01
dc.date.copyright2013-07-26
dc.date.issued2013
dc.date.submitted2013-06-28
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dc.identifier.urihttp://tdr.lib.ntu.edu.tw/jspui/handle/123456789/62529-
dc.description.abstract本研究以千年桐的未成熟、成熟種子,經過1%次氯酸鈉消毒10分鐘,置於MS培養基,在25℃光照16小時、光度28μEm-2s-1下,可100%發芽成無菌苗。將無菌苗之莖段切成0.5~1.0cm,置入MS添加4mg/l BA中4週,可誘得綠色癒合組織,再將其切取0.5cm3放入MS添加4mg/L BA與0.1mg/L IBA,光照16小時,8週後可誘得97%多芽體。
  切取無菌苗之根,置於MS添加4mg/L BA,光照16小時,4週後,每一培殖體可誘導48.2個體胚;如繼代於同樣培養基,在相同培養下,可產生二次體胚;將體胚置於添加0.1mg/l IBA培養基中,可促進體胚成熟及轉換率。
  另取2.0mg/l綠色硬實的癒合組織,置入含50ml液態培養基中,每7天以舊液:新液=1:5進行繼代,1個月後增殖為3.3mg/L ,且有細胞質濃密之細胞團出現。
zh_TW
dc.description.abstractThe Mature and non-mature seeds of Aleurites montana were used in this study, after arterialized with 1% sodium hypochlorite solution for 10 minutes. The seeds were cultured in MS culture medium, treated at 25℃ with a photoperiod of 16 hours and a light intensity of 28μEm-2s-1,which would result in 100% aseptic seedling. Cutting the stem of aseptic seedling into a length of 0.5~1.0 cm, cultured the samples in MS culture medium with 4mg/IBA for 4 weeks, which could induce the green callus, then taking 0.5cm3 sample from the green callus, cultured the sample in MS culture medium with 4mg/IBA, treated with a photoperiod of 16 hours, which could induce 97% multi-buds after 8 weeks.
Cutting roots from the aseptic seedlings, the roots were cultured in MS culture medium with 4mg/IBA, treated with a photoperiod of 16 hours, after 4 weeks, each explants could induce 48.2 somatic embryos, if sub-cultured in the same culture medium and with the same treatment, which could produce secondary somatic embryo; putting somatic embryo in the culture medium with 0.1mg/IBA, which would promote the maturation of somatic embryo and conversion ratio.
Taking 2.0mg/l green and tight callus, putting in 50ml liquid culture medium, in every 7 days, it was sub-cultured under the conditions of old liquid : new liquid = 1:5, which would increase to 3.3mg/l, and appear the formation of cell with dense cytoplasm.
en
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dc.description.tableofcontents表目次…………………………………………………………………………….……I
圖目次…………………………………………………………………………...……II
中文摘要…………………………………………………………………………V
英文摘要………………………………………..……………………………………VI
縮寫字……………………………………………...…………………………………VII
第一章 前言…………………………………...……………………………….1
第二章 前人研究……………………………………...…………………………….3
第一節 植物生長調節劑…………………………...…………………………3
第二節 器官發生…………………………...…………………………………5
第三節 癒合組織誘導…………………………...…………………………..…6
第四節 體胚發生…………………………...…………………………………7
第五節 玻璃質化…………………………...………………………………8
第六節 同科植物-麻瘋樹介紹…………………………………...……………8
第三章 材料與方法……………….………………………………………….10
第一節 材料…………………….……………………………………………10
第二節 方法……………………..…...……...……………..…………………10
2.1 種子表面消毒…………………...……...…………………..…10
2.2 基礎培養基………………………...…...…………………..…11
2.3 植物生長調節劑…………………....…..…………………..…11
2.4 細胞懸浮培養……………………..……...………………..……11
2.5 石蠟切片…………………...…………………………………..……12
第四章 結果與討論…………………………...……………...……..………………13
第一節 種子表面消毒……………………..…………...……..………………13
第二節 無菌播種………………………..…...………………..………………14
第三節 癒合組織培養………………….……………...……..………………15
3.1 癒合組織之誘導………………….……………...……..…………….15
3.2 癒合組織之增殖………………….………...…...……..………..……17
第四節 多芽體之誘導……………………..…...……………..………………20
4.1 以無菌苗莖段誘導之多芽體………………….………...…….……..20
4.2 以癒合組織誘導之多芽體.…………………………………………..21
4.3 多芽體之發根…………………….………….…...……..……………23
4.4 多芽體之抽長………..………………….……………...……..……...24
第五節 細胞懸浮培養…………….….……..………….…………………...24
第六節 體胚培養………………….…………………………………….……27
6.1 以多芽體誘導之體胚………………………...…….…………….…..27
6.2 以無菌苗之根段誘導之體胚…………….…………………………..27
6.3 體胚發芽……………….……………...………………….…………..30
6.4 二次體胚之誘導………………….……………...………………...…30
第五章 結論…………………….…………………………………….………..……32
參考文獻……………………………………………………………………………..35
附錄………………………………………. …………………………….……….…..43
附錄一 Murashige & Skoog(MS) Medium…………………………………..43
附錄二 WPM medium……………………………….……………….………44
附錄三 MS培養基製備步驟……………………….………………….…….45
附錄四 WPM 培養基製備步驟……………………………………….…….46
附錄五 懸浮培養之MS培養基製備步驟……………………………….….47
附表…………………………………….….…………….……………………………………….48
附圖……………………………………………..………………………………………………….65
dc.language.isozh-TW
dc.title千年桐之組織培養zh_TW
dc.titleTissue culture of Aleurites montanaen
dc.typeThesis
dc.date.schoolyear101-2
dc.description.degree碩士
dc.contributor.oralexamcommittee廖宇賡,李明仁,林敏宜,蕭英倫
dc.subject.keyword千年桐,癒合組織,多芽體,體胚,懸浮培養,zh_TW
dc.subject.keywordAleurites montana,callus,multi-buds,somatic embryo,suspension culture,en
dc.relation.page78
dc.rights.note有償授權
dc.date.accepted2013-06-28
dc.contributor.author-college生物資源暨農學院zh_TW
dc.contributor.author-dept森林環境暨資源學研究所zh_TW
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