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Rapid propagation of phalaenopsis from floral stalk-derived leaves

机译:蝴蝶兰从花梗衍生叶片的快速繁殖

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摘要

An efficient and rapid in vitro method was developed for regeneration of Phalaenopsis using leaf segments derived in vitro from flower stalk nodes. Leaf segments of four cultivars Tinny Sunshine 'Annie', 'Taisuco Hatarot', Teipei Gold 'Golden Star', Tinny Galaxy 'Annie' cultured on Murashige and Skoog medium supplemented with N~6-benzyladenine (BA; 88.8 μM) and α-naphthaleneacetic acid (NAA; 5.4 μM) produced an average of 10-13 protocorm-like bodies (PLBs) after 12 wk. PLB proliferation was achieved on a modified Hyponex medium (1 gl~(-1) 6.5N-4.5P-19K+20N-20P-20K+2gl~(-1) peptone + 3% (w/v) potato homogenate +0.05% activated l gl~(-1) charcoal) and an optimal number of 13-18 PLBs developed from single PLB sections of different cultivars. Plantlet development was also achieved on a modified Hyponex medium. By repeated subculture of PLBs on a proliferation medium, and culturing them in the plantlet regeneration medium, plantlets could be produced continuously. Approximately 6 mo. were required from the initiation of culture to the production of plantlets for transplant to community pots.
机译:开发了一种有效且快速的体外方法,使用从花茎节体外衍生的叶片段来再生蝴蝶兰。在Murashige和Skoog培养基上培养的4个品种Tinny Sunshine'Annie','Taisuco Hatarot',Teipei Gold'Golden Star',Tinny Galaxy'Annie'的叶段,并补充了N〜6-苄腺嘌呤(BA; 88.8μM)和α-萘乙酸(NAA; 5.4μM)在12周后平均产生10-13个原球茎样体(PLB)。在改良的Hyponex培养基(1 gl〜(-1)6.5N-4.5P-19K + 20N-20P-20K + 2gl〜(-1)蛋白ept + 3%(w / v)马铃薯匀浆+0.05的条件下实现PLB增殖%的活化的l gl(-1)木炭)和从不同品种的单个PLB部分发育的最佳数目的13-18 PLB。在改良的Hyponex培养基上也可以实现小苗发育。通过将PLB在增殖培养基上重复传代培养,并在苗再生培养基中培养,可以连续生产苗。大约6个月。从培养开始到生产小苗以移植到社区盆栽都是必需的。

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