百脉根愈伤组织原生质体再生植株

百脉根无菌苗幼茎在含２．０ｍｇ／Ｌ－,２,４－Ｄ,０．１ｍｇ／Ｌ２－ｉｐ的ＭＳ培养基上诱导和继代培养愈伤组织。选取绿色松散颗粒愈伤组织分离原生质体。原生质体培养在调整珠ＫＭ８Ｐ,Ｖ－ＫＭ,ＭＳ和ＳＨ培养基上「含３００ｍｇ／Ｌ,ＣＨ,２％ＣＷ,２％蔗糖,６％葡萄糖,２．０ｍｇ／Ｌ,２,４－Ｄ,０．５ｍｇｇ／Ｌ,ＢＡ,５ｍｍｏｌ／Ｌ ＭＥＳ」,原生质体再生细胞均能分裂,并形成小愈伤组织,但以ＫＭ８０为     

党参原生质体再生植株

党参下胚轴愈伤组织原生质体在附加１．２ｍｇ／Ｌ２,４－Ｄ,０．２ｍｇ／Ｌ ＮＡＡ,０．２ｍｇ／Ｌ ＢＡＰ和０．１ｍｇ／Ｌ ＺＴ的ＭＳ,Ｃ８１Ｖ,ＤＰＤ及ＫＭ８ｐ培养基中进行液体体层培养。在ＫＭ８ｐ中获得了最高的分裂频率。葡萄糖作渗透剂优于甘露醇,两结合使用效果更好。在合适的条件下,原生质体培养３天出现第１次分裂,４周内形成大细胞团,培养６周后形成０．５－１．０ｍｍ大小的小愈伤组织。在附加２％蔗糖     

向日葵下胚轴原生质体高频率愈伤组织形成与根发生

向日葵籽苗下胚轴原生质体,培养在含有ＢＡ０．５ｍｇ／Ｌ,２,４－Ｄ０．５ｍｇ／Ｌ,ＮＡＡ０．１ｍｇ／Ｌ和葡萄糖０．５５ｍｇ／Ｌ的改良Ｋａｏ培养基中,２４～２８ｈ后,原生质体开始分裂。包埋在琼脂糖０．６％中的原生质体,培养５ｄ后,分裂频率达９５％以上。生长旺盛的小愈伤组织转移到含有２ｉｐ０．１ｍｇ／Ｌ,ＩＡＡ０．０１ｍｇ／Ｌ,腺嘌呤４０ｍｇ／Ｌ和ＧＡ３０．０１ｍｇ／Ｌ的Ｔｈｏｍｐｓｏｎ液体培养基上１３ｄ后,原生质体诱导的少数愈伤组织发生根分化。     

杨树新品种叶肉原生质体培养和植株再生

从１ 个月龄的ＮＬ－８０１０６ 杨（Ｐｏｐｕｌｕｓｄｅｌｔｏｉｄｅｓ×Ｐ． ｓｉｍ ｏｎｉｉ）无菌苗叶片分离得到大量原生质体,纯化后其原生质体产量为４×１０７／ｇ ｆｒ．ｗ ｔ． 纯化的原生质体在含２,４－Ｄ ２ ｍ ｇ／Ｌ、ＮＡＡ ０．５ ｍ ｇ／Ｌ和ＫＴ ０．５ ｍ ｇ／Ｌ的ＫＭ８ｐ 和ＭＳ培养基中进行高密度液体浅层培养,渗透势为０．４０ ｍ ｏｌ／Ｌ的ＫＭ８ｐ 培养基中原生质体分裂频率最高． 培养第５ 天观察到第一次细胞分裂,培养１０ ｄ 的分裂频率为４．５％ ,１２ 周内可形成大量的细胞团和小愈伤组织． ＮＬ－８０１０６杨叶肉原生质体在富含有机氮并以葡萄糖为碳源的培养基中具有较高的分裂频率和植板率．小愈伤组织在ｇｅｌｒｉｔｅ 固化的ＮＬＺ１ 培养基上增殖生长,３ 周后形成４—６ ｍ ｍ 结构紧密的鲜红色愈伤组织,转至ＮＬＦ分化培养基,分化成苗率为１００％ ． 待芽伸长到３ ｃｍ 时,从基部切下转至１／２ ＭＳ培养基上诱导生根,形成完整植株     

大叶紫花苜蓿愈伤组织原生质体再生植株

大叶紫花苜蓿下胚轴诱导的愈伤组织在继代培养基上生长快速,易于分散。继代第１２ｄ的愈伤组织原生质体的得率为６．５×１０７／ｇ鲜重。原生质体培养基为ＳＨ基本培养基,含有１．０ｍｇ／Ｌ２,４－０、０．５ｍｇ／ＬＢＡ、２．０ｇ／ＬＣＨ、２％蔗糖、６％葡萄糖、５ｍｍｏｌ／ＬＭＥＳ,培养密度为１．０×１０５／ｍＬ。培养至第１２ｄ时的原生质体再生细胞植板率为３．７％。由原生质体形成的小愈伤组织在含２．０ｍｇ／Ｌ２,４－Ｄ的ＭＳ固体培养基上大量增殖。增殖的愈伤组织转移至２．０ｍｇ／Ｌ２－ｉｐ＋０．１ｍｇ／ＬＮＡＡ的Ｂ５培养基上,形成体细胞胚并发育成完整植株。     

苎麻原生质体培养及植株再生

用苎麻（Ｂｏｅｈｍ ｅｒｉａ ｎｉｖｅａ）子叶诱导愈伤组织并建立悬浮细胞系． 用４．５％ 纤维素酶、０．８％ 离析酶、０．８％ 半纤维素酶的混合酶液分离悬浮培养细胞,可得到２×１０６ 个／ｇ ｆｒ．ｗｔ的原生质体．这些原生质体以海藻酸钠包埋方式培养在附加２,４－Ｄ ０．５ ｍ ｇ／Ｌ、ＫＴ ０．５ ｍ ｇ／Ｌ 的ＫＭ８ｐ 培养基中,５０ ｄ 左右可形成肉眼可见的小愈伤组织．愈伤组织经过扩增,在不同的分化培养基上可诱导芽、根的形成,再生出完整植株． 子叶原生质体则仅能进行几次有限的分裂     

水稻游离花粉培养的高频率再生植株

用二个水稻栽培品种（Ｏｒｙｚａ ｓａｔｉｖａＬＳｕｂ．ｊａｐｏｎｉｃａ．）中花１１号和盐粳的花粉处于单核靠边期的共药,经低温处理１０－２０天,在无糖培养基中预培养２－４天后游离花粉进行培养。培养基为ＫＭ８Ｐ,附加１ｍｇ／Ｌ２,４－Ｄ,１００ｍｇ／Ｌ脯氨酸,５００ｍｇ／Ｌ水解酷蛋白,９％蔗糖。培养５天,花粉进行一次分裂,１０天后分裂频率为２１．３％,２１天可见小愈伤组织形成。随即将直径为０．５－１．     

硬粒小麦单倍体原生质体培养及植株再生

由硬粒小麦（Ｔｒｉｔｉｃｕｍ ｄｕｒｕｍ Ｄｅｓｆ．）×玉米（Ｚｅａ ｍａｙｓＬ．）建立的单倍性胚性愈伤组织,在继代培养４ 个月后置于含２．０ ｍ ｇ／Ｌ２,４－Ｄ、３％ 蔗糖、２００ ｍ ｇ／Ｌ水解酪蛋白、１４６ ｍ ｇ／Ｌ谷氨酰胺和３００ ｍ ｇ／Ｌ天冬氨酸的ＭＳ液体培养基中进行悬浮培养,４ 个月后形成了生长迅速、由大小不同（０．５ ～５ ｍ ｍ ）的愈伤组织块组成的愈伤组织悬浮系。酶解试验表明,２．０％ 纤维素酶ＲＳ和０．５％ 的离析酶效果最好,而液体悬浮培养物和固体培养的愈伤组织（在酶解时用锋利的解剖刀片切成１ ｍ ｍ 左右的小块）都能释放出大量原生质体,但悬浮培养物释放出的原生质体状态较好,胞质更浓厚,用ＫＭ８ｐ 培养基以琼脂糖包埋培养方式培养时分裂频率可达５％ 左右。由原生质体再生的小愈伤组织经增殖、筛选后可获得胚性愈伤组织,将其转移至分化培养基Ⅰ（０．２ ｍ ｇ／Ｌ ２,４－Ｄ、１．０ ｍ ｇ／Ｌ ＢＡＰ、０．１ ｍ ｇ／ＬＮＡＡ、３％ 蔗糖、２００ ｍ ｇ／Ｌ 水解酪蛋白、１４６ ｍ ｇ／Ｌ谷氨酰胺和３００ ｍ ｇ／Ｌ天冬氨酸的ＭＳ固体培养基）和Ⅱ（不含２,４－Ｄ,其它成分同Ⅰ）上进行分步分化培养可再生出完整植株,分化频率约为２０％     

甘薯叶柄原生质体有效植株再生

将甘薯（Ｉｐｏｍｏｅａｂａｔａｔａｓ（Ｌ．）Ｌａｍ．）‘元气’和‘白星’（‘ＷｈｉｔｅＳｔａｒ’）的叶柄原生质体培养在含有０．０５ｍｇ·Ｌ－１２,４Ｄ和０．５ｍｇ·Ｌ－１ＫＴ的改良ＭＳ液体培养基中,３～４ｄ后细胞开始分裂。培养８～９周后,将直径达１～２ｍｍ的愈伤组织转移到添加０．０５～０．２ｍｇ·Ｌ－１２,４Ｄ和０～０．５ｍｇ·Ｌ－１ＫＴ或添加０．５～２．０ｍｇ·Ｌ－１ＮＡＡ和１．０～３．０ｍｇ·Ｌ－１ＢＡＰ的ＭＳ固体增殖培养基上使其增殖。转移３～５周后,将愈伤组织再转移到ＭＳ基本培养基或转移到添加２．０～３．０ｍｇ·Ｌ－１ＢＡＰ的ＭＳ培养基上。当进一步转移到ＭＳ基本培养基上后,从愈伤组织或从愈伤组织形成的不定根上再生出植株。‘元气’植株再生率高达６０．０％,ＷｈｉｔｅＳｔａｒ高达４３．４％。     

草木樨状黄芪单细胞培养再生植株及其影响因素的研究

从草木樨状黄芪的子叶和胚轴诱导的愈伤组织中选取结构松脆的颗粒状愈伤组织,用液体培养基Ｓ１２进行悬浮培养建立了悬浮细胞。取换液３天左右生长旺盛的悬浮系材料分离单细胞,用基本培养基Ｓ１２与不同浓度的植物血球凝集素组成的系列培养基ＭＣ１－ＭＣ６进行液体浅层静置暗培养;形成小愈伤组织后,经Ｍ３（ＭＳ＋２,４－Ｄ ２ｍｇ／Ｌ,ＮＡＡ ０．２ｍｇ／Ｌ,ＫＴ １ｍｇ／Ｌ）培养基增殖,ＭＲ２培养基诱导分化出苗,再     

Plants regenerated from mesophyll protoplasts of white mulberry

INTRODUCTIONProtoplastcultureis0neofthen1ostrapidlydevel0pingareasinp1anttissueculture,becauseofitsimportancei11plantgeneticmanipulation.However,sofar,thereareonlyafewforesttreespeciesinwhichplantregenerationfr0mprotoplastshaJsbeensuccessful,namelyLiriode…     

枸杞下胚轴原生质体培养再生植株(简报)

枸杞是我国常用的一种滋补中药,具有较高的经济价值。以枸杞茎尖、叶片、花药、胚乳为材料的组织培养均获得再生小植株。由愈伤组织分离出的原生质体培养形成了愈伤组织。最近,由叶肉原生质体培养获     

大白菜原生质体培养再生体系的优化

以栽培大白菜亲本材料河头早A、河头早B、青麻叶C、青麻叶D、石特一号9-3、石特一号11-4、玉青、运农一号等8个品种的无菌苗下胚轴为外植体游离获得原生质体,用液体浅层法将原生质体培养在含1．5mg,NAA、0．5mg／L TDZ、0．6mg／LBA、0．5mg／L 2,4-D的DPD培养基中。培养约48h,细胞发生第一次分裂。培养到第6天发生第二次分裂。约4周,形成大量细胞团和肉眼可见的小愈伤组织。当愈伤组织长到直径4mm左右时,转入分化培养基中诱导分化,在含0．05mg／L IBA的培养基中诱导生根。对影响原生质体培养与分化的多种因素进行了较为系统的研究。     

从石刁柏原生质体培养再生植株

石刁柏,又名芦笋(Asparagus officinalisL.)是百合科天门冬属植物。其栽培品种含有丰富的维生素类及蛋白质。同时,石刁柏对于某些疾病有一定的药效,因此它已成为人们所喜爱的一种高级营养蔬菜。国外已有不少关于石刁柏试管苗繁殖的报告,但至今只有Bui Dang Ha等从石刁柏枝状叶分离的原生质体得到愈伤组织,并由此愈伤组织诱导获得了再生植株。此后,未见在石刁柏的原生质体培养方面再有新的工作。在本文中,我们利     

沙打旺原生质体培养再生植株

用1%半纤维素酶,0.4%纤维素酶,0.1%果胶离析酶,CPW9M酶液分离沙打旺无菌苗下胚轴和子叶原生质体。K8P原生质体培养基悬滴培养。下胚轴原生质体形成小细胞团后用琼脂糖包埋培养,形成小块愈伤组织后转入增殖培养基M1、M2(改良MS培养基)上形成大块愈伤组织。经过两次诱导分化,在分化培养基M3(MS 0.7mg/L BA 0.2mg/L NAA),M4(MS 0.5mg/L BA 0.5mg/L KT 0.5mg/L ZT 0.2mg/L NAA)和M6(MS 3mg/L ZT 0.2mg/L IAA)上分化出苗,再生植株。由子叶分离的原生质体未能形成愈伤组织。     

茎用芥菜细胞质雄性不育系子叶原生质体培养和高效植株再生（英文）

利用茎用芥菜细胞质雄性不育系原生质体培养获得了再生植株,并研究了影响原生质体培养的因素.结果表明,子叶是茎用芥菜原生质体培养最佳的外植体,10 d苗龄的子叶原生质体在改良MS培养基上培养3 d后发生第1次细胞分裂,6 d后发生第2次分裂,3周后形成细胞团,5周后形成肉眼可见的小愈伤.培养基中缺少NAA或2,4-D都会降低愈伤组织的再生能力.在含一定浓度的NAA(0.25 mg/L)和2,4-D(0.25 mg/L)培养基上诱导的愈伤组织质地致密且有光泽,芽的分化能力高;在MS+BA l mg/L+NAA 0.2 mg/L的培养基上芽的分化频率高达近29%,再生芽在1/2MS+NAA0.1 mg/L培养基上生根,形成完整植株.     

Plants Regenerated from Mesophyll Protoplasts of Cottonwood New Clone

Poplar NL-80106 (Populus deltoides×P, simonii) mesophyll protoplasts were isolated from leaves of 30 days-old sterile shoot, with 4 × 107/g fr. wt of protoplast yield after purification. The protoplasts were cultured in KM8p and MS liquid media containing 2 mg/L 2, 4-D, 0. 5 mg/L NAA and 0.5 mg/L KT. Higher plating density and lower osmatic pressure (0.45 mol/L) were proved to be favourable to division of protoplast-derived cells. The first division initiated 5 days after culture, and the division frequency reached 4.5 % on the 10th day. A number'of cell colonies and microcalli was formed in 12 weeks. Using organic nitrates and glucose in protoplast culture medium was beneficial to increase division frequency and plating efficiency. The calli were allowed to grow to 4--6 mm in height with red colour and compact structure on the gelrite-sohdified NLZ1 proliferation medium in 3 weeks and were transferred onto NLF differentiation medium where the frequency of shoot formation could reach 100%. The 3 cm high shoots were then cut off from the callus and rooted on 1/2 MS medium.     

茎用芥菜细胞质雄性不育系子叶原生质体培养和高效植株再生

利用茎用芥菜细胞质雄性不育系原生质体培养获得了再生植株,并研究了影响原生质体培养的因素.结果表明,子叶是茎用芥菜原生质体培养最佳的外植体,10 d苗龄的子叶原生质体在改良MS培养基上培养3 d后发生第1次细胞分裂,6 d后发生第2次分裂,3周后形成细胞团,5周后形成肉眼可见的小愈伤.培养基中缺少NAA或2,4-D都会降低愈伤组织的再生能力.在含一定浓度的NAA(0.25 mg/L)和2,4-D(0.25 mg/L)培养基上诱导的愈伤组织质地致密且有光泽,芽的分化能力高;在MS+BA l mg/L+NAA 0.2 mg/L的培养基上芽的分化频率高达近29%,再生芽在1/2MS+NAA0.1 mg/L培养基上生根,形成完整植株.     

Protoplast culture and plant regeneration from Brassica carinata Braun

Protoplasts isolated from hypocotyls of three-day-old seedlings of Brassica carinata (Braun) cv R-2128 were cultured in a modified Nitsch and Nitsch liquid medium containing 13% sucrose, 0.4% Ficoll, 0.25 mg/l BA, 0.5 mg/l NAA and 0.5 mg/l 2,4-D. The density of medium caused the protoplasts and the developing microcalli to float on the surface of the liquid medium whereas all debris and lysed cells sank to the bottom of the culture plate. After 4–6 weeks developing microcalli were approximately 0.5 mm in diameter and were transferred onto MS medium containing 3% sucrose, 0.4% agarose, 200 mg/l casein hydrolysate, 5 mg/l BA and 0.5 mg/l NAA, pH 5.7. Approximately 20% of the calli transferred to this medium produced plantlets.Abbreviations BA 6-Benzylaminopurine - NAA 1-naphthaleneacetic acid - IAA indole-3-acetic acid - 2,4-D 2,4-dichlorophenoxyacetic acid - MS Murashiqe-Skoog     

Mesophyll Protoplast Culture and Plant Regeneration of Oriental Planetree (Platanus orientalis)

Large populations of mesophyll protoplasts were released from the leaves of 1.5–2 month old sterile seedlings, with a high protoplast yield (3.7× 10 6g-1FW) after protoplast purification. The purified protoplasts were cultured in a modified K8p liquid medium supplemented with 0.5 mg/L 2,4-D, 1 mg/L NAA and 0.5 mg/L BA. Higher density (1× 106/ml) in the initial culture of protoplasts is favourable to the division of cultured mesophyll protoplasts of this woody species among the densities tested. The protoplasts started to divide after 6 days of culture, and achieved 26.8% division frequency by 14 days. Sustained divisions resulted in mass production of cell colonies and small calli in 8 weeks. The calli further grew to 2–3mm on the gelrite-solidified K8 medium supplemented with 0.2 mg/L NAA aud 0.5 mg/L BA. Then, they were transferred onto the MSB proliferation medium with 0.1 mg/L NAA and 0.25 mg/L BA, where compact and cream-coloured calli were formed. Shoot formation was initiated on MSB differentiation medium coraming 0.5 mg/L IAA, 1 mg/L each of BA and ZT. It was observed that the frequency of shoot formation was about 28.7%. Whole plantlets were regenerated upon transferring 3 cm shoots to 1/2MS medium with 0.5mg/L IBA and 0.1mg/L BA, from which they were already transplanted into pots and grew well in the phytotron of Shanghai Institute of Plant Physiology.