白刺花胚性愈伤组织诱导及体细胞胚发生和萌发

探讨不同因素对白刺花下胚轴、子叶2种外植体胚性愈伤组织诱导及体细胞胚发生和萌发的影响。以B5和MS为基本培养基,研究2,4-D、6-BA和TDZ对白刺花下胚轴和子叶胚性愈伤组织的诱导;在MS培养基上添加不同浓度2,4-D,研究胚性愈伤组织增殖情况;采用ABA,探究对体细胞胚发生的影响。结果表明:下胚轴比子叶更易诱导胚性愈伤组织,筛选出2种外植最佳的胚性愈伤组织诱导培养基均为MS+2.0 mg/L 2,4-D+0.5 mg/L TDZ+0.5 mg/L 6-BA,胚性愈伤组织诱导率分别为77.3%和41.0%。15.0 mg/L ABA、0.2 mg/L 2,4-D和2.0 mg/L 6-BA有利于体细胞胚发生,1/3MS+0.2 mg/L NAA+0.1 mg/L 6-BA+2.0 g/L活性炭+25 g/L蔗糖+7 g/L琼脂的培养基可使体细胞胚萌发率达80%以上,再生植株移栽成活率高达90%。白刺花外植体种类及培养基类型均会影响胚性愈伤组织的诱导,其中下胚轴诱导效果优于子叶;MS培养基较适合启动细胞脱分化形成愈伤组织,2,4-D对胚性愈伤组织的增殖保持有调控作用,ABA有利于体细胞胚的发生。     

塔杨松散型均质胚性愈伤组织培养体系

为了获得塔杨(Populus×canadensis Moench‘Tower’)松散型、均质、胚性愈伤组织(LHEC),以塔杨试管苗叶片为外植体,通过不同浓度激素(BA、KT、2,4-D)、蔗糖和无机盐处理,建立了松散型愈伤组织(LC)诱导—继代培养—胚性愈伤诱导的高效体系。结果显示:塔杨叶片在低蔗糖和低无机盐(1/4MS+2 mg·L~(-1)2,4-D+1mg·L~(-1)BA+10 g·L~(-1))的培养基上培养可以诱导出完全的LC(诱导率100%)。LC在继代培养基(MS+2.0mg·L~(-1)2,4-D+2.0 mg·L~(-1)BA+Vc100 mg·L~(-1)+30 g·L~(-1))上进行2~3次转接后,再转移到LHEC培养基(MS+0.5 mg·L~(-1)2,4-D+3 mg·L~(-1)BA+Vc100 mg·L~(-1)+40 g·L~(-1)蔗糖)上培养4~5周(每7天转接1次),即可诱导出具有许多球状体(原胚状体)的松散型胚性愈伤组织。此外,适当的2,4-D与BA浓度比例,可以使LC保持细胞的松散特性、不形成根、无褐变,生长快;含有30 g·L~(-1)蔗糖的培养基利于LC生长和LHEC的形成;维生素C能较好的抑制继代培养中的褐变;BA有利于形成LC,而KT有利于紧密型愈伤组织的形成,同时BA处理的愈伤组织生长较KT处理的快;当2,4-D浓度为0.5~1 mg·L~(-1)时,随着BA浓度的增加,LHEC的数量也随之增加,当BA为3 mg·L~(-1)时,LHEC数量达到最大值100%。本文还对影响愈伤组织胚性化的主要因素进行了讨论。提出的各项建议对均质胚性愈伤组织LHEC的培养有重要的指导意义。     

‘宁杞8号’体细胞胚胎发生体系建立

以宁夏枸杞新品种‘宁杞8号’幼嫩叶片为外植体,探讨激素组合及添加物对‘宁杞8号’体细胞胚胎诱导、体胚增殖、萌发和植株再生的影响,并建立高效稳定的体细胞胚胎发生体系。结果表明:通过对6-BA、2,4-D和IAA进行正交分析,筛选出‘宁杞8号’体细胞胚诱导最优激素组合:6-BA 1.0 mg·L~(-1)+2,4-D0.3 mg·L~(-1)+IAA 0.4 mg·L~(-1),体胚诱导率达88.67%。极差分析比较各激素间的影响,6-BA对体胚诱导影响最显著。当高浓度的生长素及低浓度细胞分裂素浓度适宜的配比时,才能诱导产生形态正常数量多的‘宁杞8号’体细胞胚。在体胚增殖培养中,6-BA的浓度过高易导致玻璃化,不利于‘宁杞8号’体胚增殖生长。随着激素浓度的增高,体胚增殖倍数增加,玻璃化率也越高,综合分析得到‘宁杞8号’最佳体胚增殖培养基为6-BA 0.4 mg·L~(-1)+NAA 0.6 mg·L~(-1)。当添加IBA 0.3 mg·L~(-1)+GA_30.4 mg·L~(-1)+蔗糖10 g·L~(-1)时,‘宁杞8号’体胚萌发率最高,萌发率达89.17%。添加GA_3及低浓度蔗糖能促进成熟的体胚萌发。对‘宁杞8号’体萌发的影响程度依次是IBA蔗糖GA_3。活性炭能有效提高‘宁杞8号’体胚再生植株率,同时对萌发体胚的根的发育也有促进作用,当IBA 0.1 mg·L~(-1)+KT 0.4 mg·L~(-1)+活性炭1 g·L~(-1)时,‘宁杞8号’体胚再生植株效果最佳,体胚再生率达91.67%。     

绒毛白蜡体胚诱导和植株再生

该文探讨了基本培养基、外植体、培养条件以及植物生长调节剂配比对绒毛白蜡(Fraxinus velutina)体胚诱导的影响。结果表明,胚根是诱导体胚发生的最佳外植体;体胚诱导的最适培养基为改良MS+2 mg·L~(–1) 6-BA+0.1 mg·L~(–1) NAA、30g·L~(–1)蔗糖、5.0 g·L~(–1)琼脂;暗培养20天后进行光照培养(14小时光照/10小时黑暗),光密度为100~(–1)20μmol·m~(–2)·s~(–1),昼温度(25±2)°C,夜温度(18±2)°C;成功诱导出体细胞胚并获得再生植株,体胚诱导率可达59.8%,体胚萌发率达81.2%。壮苗最适培养基为改良WPM+0.5 mg·L~(–1) 6-BA+0.2 mg·L~(–1) ZT+0.01 mg·L~(–1) NAA。生根最适培养基为改良1/2MS+1.0 mg·L~(–1)IBA+0.05 mg·L~(–1) NAA+20 g·L~(–1)蔗糖,生根率高达97.3%,试管苗移栽成活率达97.8%。     

‘SK4—316’胡萝卜体胚的诱导和培养

以'SK4-316'胡萝卜无菌苗的下胚轴为外植体,研究不同培养基配方和培养条件对愈伤组织诱导、体细胞胚间接发生及其同步化培养的影响,以及不同脱分化时间、脱分化培养基及外植体续存时间对体细胞胚直接发生的诱导及其培养的影响.结果表明:含3%蔗糖、0.8%琼脂的1/2MS + 2,4-D 2.5 mg/L + 6-BA(或KT)0.5 mg/L + CH 300 mg/L是诱导愈伤组织的良好培养基;1/2MS + 2,4-D 1.25 mg/L + KT 0.25 mg/L + 6-BA 0.25 mg/L(含3%蔗糖)适于愈伤组织分化并诱导体胚发生,0.02% ABA对体胚的诱导有促进作用,0.06% ABA或15% PEG能促进体胚成熟;外植体在MS + 2,4-D 1.0 mg/L固体培养基上脱分化培养48 h,再转入MS + CH 300 g/L液体培养基中可诱导体胚直接发生,但随着外植体续存于诱导培养基中时间的延长,体胚发生变异的几率也渐增.     

渗透剂对白刺花体细胞胚成熟及萌发的影响

该研究以蔗糖、麦芽糖、山梨醇及PEG(6000)为渗透剂,探讨了不同渗透剂对白刺花体细胞胚发育、胚成熟及萌发的影响。结果表明:白刺花下胚轴形成的胚性愈伤组织接种至MS+2,4-D 0.2 mg·L~(-1)+NAA 1.0 mg·L~(-1)+6-BA 2.0 mg·L~(-1)+TDZ 1.0 mg·L~(-1)+蔗糖40 g·L~(-1)+谷氨酰胺100 mg·L~(-1)+植物凝胶3g·L~(-1)的培养基上,体细胞胚发生率高达66. 21%,总胚数为79个; 7%蔗糖可使体细胞胚成熟率高达64.36%,同时也可提高多子叶畸形胚形成; 2%麦芽糖+2%山梨醇+4%蔗糖组合使体细胞胚成熟率最高达88.89%,畸形胚比例最低; 30 g·L~(-1)PEG培养时,体细胞成熟率最高,为82.35%;鱼雷期的体细胞胚最合适转接,可使体胚萌发率达90.58%,复合糖上培养得到的成熟体细胞胚生根率最高,为87.47%。这为实现白刺花体细胞胚育苗奠定了理论基础,并提供了可行的方案。     

文冠果的体细胞胚胎发生

文冠果种子在MS 6-BA 1.0 mg·L-1 2,4-D 1.0 mg·L-1 NAA 1.0 mg·L-1 3%蔗糖的固体培养基上暗培养,形成愈伤组织,愈伤组织在B5 6-BA0.5mg·L-1 NAA0.5mg·L-1 2%蔗糖的培养基中弱光悬浮培养形成体细胞胚.在蔗糖为1%时,子叶状胚萌发形成完整小植株.细胞学观察表明,文冠果体细胞胚源于胚性愈伤组织的外层细胞,此区域细胞富含淀粉粒.     

红花草莓的组织培养与快繁技术研究

以红花草莓叶片为外植体,通过筛选诱导愈伤组织、不定芽及壮苗、生根的培养基,建立一套实用且易推广的红花草莓组培快繁技术体系。结果表明:在愈伤组织的诱导过程中TDZ的诱导效果优于6-BA,TDZ与NAA配合使用效果优于与IBA的组合。6-BA浓度为0.5 mg·L~(-1)时不定芽诱导率高达86.6%。低浓度的6-BA和8 g·L~(-1)的琼脂更有利于壮苗培养,NAA比IBA更有利诱导生根。综上述,最适红花草莓愈伤组织的诱导培养基为MS+1.0 mg·L~(-1)TDZ+0.5 mg·L~(-1)NAA+30 g·L~(-1)蔗糖+7 g·L~(-1)琼脂;最适不定芽分化的培养基为MS+0.5 mg·L~(-1)6-BA+0.1 mg·L~(-1)NAA+30 g·L~(-1)蔗糖+7 g·L~(-1)琼脂;最适壮苗培养基为MS+0.1 mg·L~(-1)6-BA+0.1 mg·L~(-1)NAA+30 g·L~(-1)蔗糖+8g·L~(-1)琼脂;最适生根培养基为MS+0.5mg·L~(-1)NAA+30 g·L~(-1)蔗糖+8 g·L~(-1)琼脂。试管苗移栽生长20 d后,成活率高达93%,且后期草莓苗生长壮健。此体系的建立为优质红花草莓种苗大规模生产提供了科学依据和技术支持。     

中粒种咖啡花药培养成完整植株

1 植物名称中粒种咖啡(coffea robusta)。 2 材料类别花药。 3 培养条件基本培养基为MS,(1)诱导愈伤组织培养基附加KT0.8 mg/L(单位下同)、2,4-D 0.8、NAA1、蔗糖5％、琼脂0.5％,pH 5.8。(2)诱导胚状体培养基附加BA 2、KT 0.5、NAA 0.2、CH 500、蔗糖3％、琼脂0.6％,pH 5.8。(3)胚状体分化成苗培养基为3/4MS附加BA0.5、NAA0.8、GA0.1、活性炭0.1％、蔗糖2.5％、琼脂0.7％,pH 5.8。培养温度25     

陇东地区野生紫花苜蓿植株再生体系的建立

以陇东地区野生紫花苜蓿无菌苗的下胚轴、子叶、叶片和叶柄为外植体,MS为基本培养基,研究划破种皮以及不同生长调节物质种类与配比对愈伤组织诱导和分化影响的结果表明：划破种皮可提高种子发芽率;在外植体中下胚轴的愈伤组织诱导率最高,达92.2%;最佳愈伤组织诱导培养基为MS＋2,4-D2.0mg·L^-1（单位下同）＋NAA1.0＋2.5%蔗糖＋0.6%琼脂,最佳分化诱导培养基为MS＋KT0.5＋NAA0.3＋2.5%蔗糖＋0.6%琼脂,成苗培养基为1/2MS＋NAA0.1＋1%蔗糖＋0.6%琼脂。     

黄山栾树体细胞胚的发生和组织学观察

黄山栾树无菌苗的节间和叶柄离体培养后,其体细胞胚发生的结果表明：节间愈伤组织可诱导产生体细胞胚,而叶柄愈伤组织则生根：节间愈伤组织诱导培养基为MS＋3．0mg．L～2,4．D＋0．5～3．0mg．L-1NAA;节间胚性愈伤组织诱导培养基为MS＋2．0nag．L-2,4-D;胚性愈伤组织转移到无植物生长调节剂的MS培养基上可发育成正常植株。组织学观察表明,体细胞胚在胚性愈伤组织中有的发生于愈伤组织表层细胞,有的发生在愈伤组织内部。黄山栾树体细胞胚的形成经历球形胚、心形胚、鱼雷胚和子叶胚几个阶段,这与合子胚的发育途径相似。     

花生体细胞胚的诱导及其植株再生

采用不同成熟度的花生胚轴为外植体进行体细胞胚诱导及植株再生研究,结果表明,成熟胚轴在高浓度2,4－D的MS培养基中,经过30d左右的培养,可直接诱导产生出大量的体细胞胚,含40mgL~－12,4－D的培养基中体细胞胚的诱导率达100％,平均每个外植体产生11．58个体细胞胚．体细胞胚的继代培养需降低2,4－D的浓度（1－20mgL~－1）．未成熟胚轴的体细胞胚诱导及继代培养的2,4－D浓度宜为10mgL~－1．将诱导的体细胞胚转接到合5－10mgL~－1BA的MS培养基中,体细胞胚能够萌发再生成无根小植株,将其转接到生根培养基中可获得完整小植株．     

Primary and repetitive secondary somatic embryogenesis in <Emphasis Type="Italic">Rosa hybrida</Emphasis> ‘Samantha’

This study describes a plant regeneration system for Rosa hybrida ‘Samantha’, a mainstream commercial cultivar, via direct somatic embryogenesis. Somatic embryogenesis was induced from in vitro-derived leaf explants, achieving a frequency of 7.5% following 8 weeks of culture on a Murashige and Skoog (MS) medium supplemented with 3.0 mg/L 2,4-dichlorophenoxyacetic acid (2,4-D) and 30 g/L glucose. We evaluated the effects of various types and concentrations of carbohydrates and plant growth regulators (PGRs) on the proliferation and germination of secondary somatic embryos. MS medium containing 1.0 mg/L 2,4-D, 0.05 mg/L 6-benzyladenine (BA) and 60 g/L glucose was found to be the most effective in promoting the proliferation of somatic embryos. The highest germination rate (56.2%) of somatic embryos was observed on MS medium containing 1.0 mg/L Thidiazuron (TDZ) and 0.5 mg/L BA. Whole plantlets were obtained by culturing germinated shoots on rooting medium comprising 1/2-strength MS salts supplemented with 0.05 mg/L α-Naphthalene acetic acid (NAA). Plantlets grew vigorously with normal vegetative and flowering characteristics.     

领春木体细胞胚胎发生及植株再生

以领春木（Eupteleapleiospermum Hook．f.etThoms．）种子幼胚为试验材料,对领春木体细胞胚胎发生进行了研究。结果表明：在附加1．0mg·L-1 2,4．D＋0．5mg·L-1 6-BA＋3％蔗糖＋0．8％琼脂的Ms培养基上可诱导出愈伤组织。愈伤组织在附加0．5mg·L-1 NAA＋0．5mg·L-1 6．BA的培养基上可形成体细胞胚;体胚在附加0．5mg·L-1 6-BA＋0．05mg·L-1 NAA＋0．1％PVP的1／2MS培养基上能大量增殖;将成熟体胚转移到不添加任何植物生长调节剂的MS培养基上,培养60d,形成正常植株。     

Development of in vitro plant regeneration of Australian native waxflowers (Chamelaucium spp.) via somatic embryogenesis

Waxflowers (Chamelaucium spp.) are native to Australia and now are grown for the cut flower industry worldwide. As part of an effort to achieve somatic hybridization between the species to improve flower quality, somatic embryogenesis was achieved for Chamelaucium uncinatum and C. repens. Somatic embryos from young leaves of C. uncinatum and C. repens were induced in vitro on Murashige and Skoog (MS) agar medium containing 20 g/l sucrose and 2,4-dichlorophenoxyacetic acid (2,4-D). For C. uncinatum, up to 4% of explants developed somatic embryos at 20 μM 2,4-D and for C. repens, up to 3% developed somatic embryos at 5 μM 2,4-D. Somatic embryos of C. uncinatum were also induced from immature seeds—a maximum of 6% of seed explants producing somatic embryos on MS medium containing 0.05 μM 6-benzyladenine (BA) and 0.5 μM Naphthalene acetic acid (NAA). Somatic embryo cultures maintained on MS medium supplemented with 0.1 μM 2,4-D were induced to develop into plantlets after transfer to a hormone-free medium under light.     

扁蓿豆体细胞胚的诱导和植株再生

扁蓿豆实生苗的根、下胚轴、子叶、叶片和叶柄外植体,在含２,４—Ｄ２—０．２５ｍｇＬ－１与ＫＴ０．２５－２ｍｇＬ－１及２,４—Ｄ０．５ｍｇＬ－１与ＺＴ０．５ｍｇＬ－１或ＢＡＰ０．５ｍｇＬ－１与ＮＡＡ０．０５ｍｇＬ－１的ＭＳ琼脂培养基上均可产生愈伤组织．愈伤组织在含２,４—Ｄ０．５—０．１ｍｇＬ－１与ＫＴ０．５—０．１ｍｇＬ－１或ＢＡＰ０．２５＋ＮＡＡ０．０５ｍｇＬ－１的ＭＳ培养基上可诱导分化出体细胞胚．体细胞胚在无激素的培养基上发育成完整植株．用海藻酸钠包襄体细胞胚制成人工种子,其发芽率和植株转换率分别为９５％和５３％．     

High Frequency Plant Regeneration from Astragalus melilotoides hypocotyl and stem explants via somatic embryogenesis and organogenesis

An efficient and reproducible procedure is established for the plant regeneration from hypocotyl explants and hypocotyl-or stem-derived calli in Astragalus melilotoides. High frequency somatic embryo formation (98.3%) occurred direct on hypocotyls on Murashige and Skoog (MS) medium supplemented with 2.69 µM NAA and 4.44 µM BA within 5 weeks. Three types of calli were induced from the hypocotyl and stem segments on MS medium containing 9.05 µM 2,4-D and 2.22–4.44 µM BA. Both somatic embryos and adventitious buds were initiated from hypocotyl-derived calli while only adventitious buds were formed from stem-derived calli in MS medium supplemented with 2.69 µM NAA and 4.44–8.89 µM BA. Somatic embryos or adventitious buds developed into plantlets following being cultured for 3 weeks on MS medium without any growth regulators or with 14.78 µM IBA, respectively. All the regenerated plants were normal with respect to morphology and growth characters, and produced fertile seeds after planting in soil.     

深山含笑的组织培养和快速繁殖

组织培养深山含笑的实验结果表明：利用休眠芽和种子萌发时实生苗的上胚轴及下胚轴为外植体均能诱导出愈伤组织和不定芽,其中无菌实生苗的上胚轴最易诱导出不定芽,无菌实生苗的下胚轴最易诱导出愈伤组织。外体植体在ＭＳ＋１．０－２．０ｍｇ Ｌ＾－１ ２,４－Ｄ培养基上只产生愈伤组织;在ＭＳ＋３．０ｍｇ Ｌ＾－１ ＢＡ＋０．２ｍｇ Ｌ＾－１ ＮＡＡ培养基上产生较多的不定芽和较多的愈伤组织;在ＭＳ＋２．０ｍｇ Ｌ＾     

杂交兰类原球茎增殖中芽分化的控制和快速繁殖

以‘玉女杂交兰’为材料,研究了培养时间、活性炭、切块大小和外源生长调节物质对类原球茎增殖和分化的影响。结果表明,培养时间、活性炭和切割处理对类原球茎增殖和分化影响显著,在培养基中添加活性炭或对类原球茎进行切割均能有效控制增殖过程中的芽分化。将类原球茎切成直径2~3 mm的小块接种到培养基MS＋1.0 mg.L-16-BA＋0.2 mg.L-1NAA＋0.3 g.L-1AC＋30 g.L-1蔗糖＋5.5 g.L-1琼脂中培养40 d,类原球茎增殖率为384.23%。将增殖后的类原球茎接种到培养基1/2MS＋1.5 mg.L-16-BA＋0.1 mg.L-1NAA＋20 g.L-1蔗糖＋5.5 g.L-1琼脂中培养40 d,芽分化率为463.06%。将分化的芽转入培养基1/2MS＋0.5 mg.L-1NAA＋0.5 g.L-1AC＋20 g.L-1蔗糖＋100 g.L-1土豆汁＋5.5 g.L-1琼脂中培养,生根率为100%,平均根分化数为2.80条.株-1。以泥炭土为基质,组培苗的移栽成活率可达97.78%。     

<Emphasis Type="Italic">In vitro</Emphasis> propagation of <Emphasis Type="Italic">Ophiorrhiza prostrata</Emphasis> through somatic embryogenesis

In vitro propagation of an anticancerous drug synthesizing plant, Ophiorrhiza prostrata D. Don, was established through indirect somatic embryogenesis. Friable embryogenic calluses were initiated from O. prostrata leaf and internode explants on Murashige and Skoog (MS) media supplemented with 2,4-dichlorophenoxyacetic acid (2,4-D) either alone or in combination with N⁶-benzyladenine (BA) or kinetin (KIN). Somatic embryos were developed after subculture of the friable calluses onto half strength MS media containing 0.45 or 2.26 μM 2,4-D alone or in combination with BA or KIN. Medium supplemented with 2.26 μM 2,4-D and 2.22 μM BA was optimal, supporting the production of a mean of 5.8 globular embryos. Subculture of globular embryo-bearing calluses on half strength MS medium without growth regulators produced the highest embryo frequency, and the majority of them developing to early torpedo stage. Somatic embryos underwent maturation and converted to plantlets at high frequency (90 %) on half strength MS medium supplemented with 0.44 μM BA. Somatic embryo-derived plantlets with well-developed roots were established in field conditions with a 90 % survival rate.