紫斑牡丹胚培养与植株再生（简报）

紫斑牡丹专性种子繁殖,效率极低。通过胚培养,种胚在1／2MS＋BA1．0mg/L(单位下同）＋IAA1．0培养基上可以较快生长并分化出不定芽,不定芽在1／2MS＋BA1.0 IAA0.2培养基上可实现快速增殖,40d平均增殖倍数为6．5,增殖芽在1／2MS＋IAA0．2培养基上可快速高效生根。     

枣叶片离体培养再生植株

PlantletRegenerationfromLeavesCulturesofZizyphusiuiubaCHENZong－Li,YANZhi－Lian,QILong（Denyt17mllofmp,You’onl／nll＊,ndy,Yan’as716000）1植物名称枣（凯W…。Wwi）。2材料类别俗名“狗头枣”的无菌试管苗的叶片。3培养条件（l）叶片愈伤组织诱导及继代培养基：MS＋6－BA0．3mg／L（单位下同）＋2,4D20;（2）芽分化培养基：MS＋6－BAI．0＋IBA0．2＋D一泛酸钙1．0十活性发0．5％;（3）芽生长培养基：1／2MS＋6－BA0．2＋IAA0．04＋D一泛酸钙1．0;（4）芽增殖培养基：1／2MS＋6－BA0．4＋IAA0．0…     

龙须海棠组织培养与试管内开花

1植物名称龙须海棠（Mesembryanthemum spectabileFlaw）。2材料类别种子。3培养条件种子萌发培养基：（1）1/2MS;增殖继代培养基：（2）MS＋6-BA2.0mg·L^-1（单位下同）＋NAA0.2;（3）MS＋6-BA1.0＋NAA0.5;（4）MS＋6-BA0.5＋NAA0.1;生根培养基：（5）1/2MS＋NAA0.1;（6）1/5NAA0．1;生根培养基：（5）1／2MS＋NAA0．1;（6）1／5MS＋NAA0．I＋PP3330．1。     

绿巨人茎尖的离体培养及快速繁殖

1植物名称绿巨人（SpathiphyllumKochii）。2材料类别带顶芽茎段经表面消毒后从顶端分离出的2mm茎尖。3培养条件培养基：（1）1／2MS＋6－BA0．1mg·L－1（单位下同）＋IAA0．3;（2）MS＋6－BA0．5＋NAA0．5;（3）1／2MS＋6－BA0．1＋IBA0．5。以上培养基均含3％蔗糖、0．8％琼脂,pH5．8。培养温度28～30℃,照光12h·d－1,光照度2000lx。4生长与分化情况4．1茎尖的制备与培养从盆栽的生长旺盛、粗壮无病虫害的绿巨人植株上切取4cm带顶芽的茎段,除去叶片和大部分叶柄后,置烧杯中,加入1滴中性洗涤液及少量自来水,用细软的…     

液体悬浮培养促进铁皮石斛原球茎高效诱导、增殖的研究

用正交设计方法对铁皮石斛原球茎具有高效增殖影响的激素（BA,NAA,KT,马铃薯汁）以及配比进行研究,结果表明：以茎段为外植体在培养基Ms＋BA2．0mg／L＋NAA2．0mg／L＋马铃薯汁10％＋糖3％,具有很好的原球茎诱导作用,50d后诱导率达95．20％;原球茎在1／2MS＋BA2．0mg／L＋NAA1．0mg／L＋KT0．5mg／L＋糖3％的培养基上,以液体悬浮培养,原球茎增殖达49．032g／50d。     

三倍体枇杷的茎尖培养及诱导生根

以三倍体枇杷为材料, 研究了不同消毒方式、MS培养基浓度、植物生长调节剂及浓度配比对茎尖培养及诱导生根的影响。结果表明, 初代培养时, 选择生长饱满、健壮的顶芽及适宜的消毒方式, 外植体剥离长度0.5-0.8 cm, 能显著提高茎尖培养的成活率; MS培养基浓度的变化对外植体的褐化没有明显的影响; 最适茎尖的启动培养基为MS＋1.0 mg·L-1 6-BA＋0.5 mg·L-1 NAA, 成活率高达84.8%; 最适组培苗生根培养基为1/2MS＋0.1 mg·L-1 NAA＋0.01 mg·L-1 IAA＋0.3%活性炭, 生根率达66.7%, 每株平均生根2.83条。该研究结果将为三倍体枇杷再生体系的建立及利用转基因技术对三倍体无籽枇杷进行遗传改良奠定基础。     

芋茎尖离体培养和快速繁殖

对芋优良品种莱阳毛羊头进行茎尖培养和快速繁殖。试验表明,外植体表面灭菌的最佳方案是乙醇→新洁尔灭→剥幼叶→升汞。在较软的培养基中,茎尖大于0．6mm,成活率为90％以上。不定芽分化的最适培养基为MS＋BA1（mg／L以下单位相同）＋NAA0．2＋Spm20,其分化率为100％。不定芽在MS＋BA2＋NAA0．1＋Spm50的培养基中,可实现继代繁殖和诱导生根一步完成,月增殖系数达7．3,生根率88．3％。芋试管苗移栽于沙壤土基中,成活率为90％以上,且生长健壮,根系发达。     

人参发根的诱导及其适宜培养条件的研究

利用发根农杆菌A₄菌株在人参根外植体上直接诱导产生发根。在1/2MS固体培养基上建立起发根离体培养系,经连续多代的培养,发根仍保持旺盛生长状态。PCR扩增结果表明,发根农杆菌R_I质粒的rolC基因已在人参发根基因组中整合并得到表达。液体培养基中发根生长速度约为固体培养的2倍。经对发根中人参皂苷含量及比生长速率的测定,筛选出高产发根系R9923。利用HPLC法测定了R9923发根系中单体皂苷Rg1、Re、Rf、Rb1、Rc、Rb2和Rd的含量,人参总皂苷含量达15.2mg/g。确定1/2MS培养液（30g/L蔗糖）、摇床转速110r/min、每２周更换一次培养液、继代培养时间4周,为人参发根生长适宜条件。探讨了培养容积、发根初始接种量以及分级放大培养工艺对发根大规模生产过程中生物产量和皂苷含量的影响。     

水浮莲无菌苗的获得及其培养体系的优化

为了有效地进行水浮莲（Pistia stratiotes）的基因工程改造,达到利用水浮莲进行污染水体的植物修复,本研究建立了水浮莲无菌苗培养体系。采用二次消毒法获得水浮莲的无菌苗,并研究了萘乙酸（NAA）、6-苄氨基嘌呤（6-BA）、蔗糖、pH值对其生长的影响,确立了水浮莲的优化培养体系为：1/2 MS＋6-BA 0.25mg/L＋NAA 0.3mg/L＋蔗糖20g/L,pH6.0。水浮莲在此培养基上可快速扩增和长期继代培养,无菌生长的水浮莲比温室中自然水浮莲的植株形态小,易于研究操作。     

八宝剑凤梨的组织培养与快速繁殖

TissueCultureandRapidPropagationofVrieseapoelmaniiZHONGHong-Mei;CAOMing-Hua（AzollaResearchCentre,FujianAcademyofAgriculturualSciences,Fuzhou350013）1植物名称八宝剑凤梨（Vrieseapoelmanii）。2材料类别侧芽。3培养条件（1）丛生芽诱导培养基：MS＋6－BA2mg·L(-1)（单位下同）＋NAA0．2,试管内滤纸桥液体培养;（2）增殖培养基：MS＋BA1＋NAA1,浅层液体培养;（3）生根培养基：1／2MS＋NAA0．1－0．2＋0．7％琼脂。上述培养基均含3％的蔗糖,pH5．6。培养温度23～26℃,光照度1500－2000lx,每天光照1…     

贯叶金丝桃组织培养的研究

分别以甘肃天水贯叶金丝桃的幼根、幼茎、幼叶为外植体．在1／2MS培养基上附加各类激素,进行贯叶金丝桃的组培实验。研究发现各外植体的增殖速率由高到低分别为幼茎、幼根、幼叶,且得到贯叶金丝桃组培各阶段的最佳培养基成分。诱导愈伤组织的培养基为1／2MS 1．3～1．6mg／L BA 0．2mg／L NAA;培养基1／2MS 1．3～1．6mg／L BA 0．15mg／L NAA有利于不定芽的形成;诱导不定根的培养基为l／2MS IBA0．5～O．8mg／L 蔗糖2．0％。向1／2MS培养基中添加不同的生长素(IAA,IBA,NAA,2．4-D)．在不同浓度梯度的培养基上进行诱导贯叶金丝桃的愈伤组织及不定根的试验,结果表明：生长素IAA,IBA既可诱导愈伤组织,又可以诱导不定根的产生。生长素NAA,2,4-D可诱导产生愈伤组织,但对不定根的诱导作用较差。     

美洲商陆毛状根诱导及其离体培养的影响因素

为了探讨利用美洲商陆毛状根生产其药用成分的可能性,研究了美洲商陆毛状根诱导及其离体培养的影响因素。结果表明,美洲商陆叶片外植体被发根农杆菌ATCC 15834感染约18 d后,从其叶片外植体形态学下端叶脉切口处产生毛状根,其中以预培养1 d,农杆菌感染20 min,共培养4 d时的毛状根诱导率最高,达到70%。PCR扩增和硅胶薄层层析结果显示,发根农杆菌Ri质粒的rol C基因以及冠瘿碱合成酶基因已在美洲商陆毛状根基因组中整合和表达。所获得的美洲商陆毛状根系都能在无外源激素的MS固体培养基上快速自主生长;其中以毛状根根系2的生长速度最快、分生侧根能力最强和根表面的根毛密度最高;毛状根根表面呈紫红色或呈白色。在供试的MS、1/2MS、B5和6,7-V液体培养基中,以无外源激素的MS培养基最适合美洲商陆毛状根根系生长。与无外源激素的MS培养基相比,6,7-V培养基更有利于毛状根中商陆皂苷甲的合成与积累。本文所建立的美洲商陆毛状根诱导及其离体培养的适宜条件为今后利用其毛状根株系的规模培养来生产其药用有效成分商陆皂苷甲奠定了实验和技术基础。     

烟草毛状根诱导及其茄尼醇含量初探

茄尼醇是合成泛醌类药物的重要中间体。以发根农杆菌(Agrobacterium rhizogenes)W.T15834感染烟草叶片诱导产生毛状根, 探讨其茄尼醇含量变化。结果显示, 获得的毛状根能在无外源生长调节剂的MS固体和液体培养基上自主生长, 但在液体培养基中培养的毛状根生长更迅速, 也不会形成愈伤组织。甘露碱检测及PCR结果证实, 发根农杆菌Ri质粒的rolB基因已在烟草(Nicotiana tabacum)毛状根基因组中整合并得到表达。用改进的HPLC法测定烟草毛状根中的茄尼醇含量, 其结果为对照根(种子萌发产生的幼苗根)的1.12倍, 但仍比废弃烟叶中茄尼醇含量低43.2％。     

烟草毛状根诱导及其茄尼醇含量初探

茄尼醇是合成泛醌类药物的重要中间体.以发根农杆菌（Agrobacterium rhizogenes）W.T15834感染烟草叶片诱导产生毛状根,探讨其茄尼醇含量变化.结果显示,获得的毛状根能在无外源生长调节剂的MS固体和液体培养基上自主生长,但在液体培养基中培养的毛状根生长更迅速,也不会形成愈伤组织.甘露碱检测及PCR结果证实,发根农杆菌Ri质粒的rolB基因已在烟草（Nicotiana tabacum）毛状根基因组中整合并得到表达.用改进的HPLC法测定烟草毛状根中的茄尼醇含量,其结果为对照根（种子萌发产生的幼苗根）的1.12倍,但仍比废弃烟叶中茄尼醇含量低43.2%.     

In vitro direct rhizogenesis from Gerbera jamesonii Bolus leaf

The present report describes an original protocol for in vitro direct induction of roots from leaf explants of gerbera for the first time. Since gerbera has immense potential as a premium cut-flower, the major attempts were made on in vitro mass propagation chiefly through in vitro multiple shoot proliferation or callus regeneration. Nevertheless, rhizogenesis could be impending an unattempted method with its yet-to-be known advantages. In our study, the optimum conditions for direct root induction from leaf explants were assessed employing tissue culture technique. Leaves were inoculated to MS medium containing no or variable auxin sources and concentrations namely, 2,4-dichlorophenoxyacetic acid, indole-3-acetic acid (IAA), indole-3-butyric acid or α-naphthaleneacetic acid for root induction. It was evident that the maximum root induction (with a frequency of 92.6 %) occurred on MS media fortified with 1.5 mg l^?1 IAA, wherein root induction was observed as early as 11 days of culture and an average of ~19 roots with ~13 mm length was obtained from 4 cm² leaf segment after 45 days of culture. Stereo microscopic observation revealed the induction of roots and gradual developmental stages of rhizogenesis. The efficiency of direct root induction without any interim growth stages (such as, callus or shoots) in our study offers a reproducible system that could provide a model protocol for more comprehensive developmental studies on root growth.     

“艾西丝”南瓜诱导生根过程中过氧化物酶活性及同工酶的研究

以“艾西丝”南瓜组培苗为材料,研究其在诱导不定根形成过程中过氧化物酶活性及同工酶谱的变化。结果表明,当南瓜无根苗从含有较高浓度的ＢＡ培养基转入１／２ＭＳ培养基后,可诱导无根苗茎基部不定根生成,一般在转入生根培养基第３ｄ开始生根,至第６ｄ生根率达７０％以上。在此期间,南瓜茎内过氧化物酶活性由低增高,即在不定根形成之前,过氧化物酶活性处在较低水平,而当不定根形成时,过氧化物酶活性迅速升高,以后一直维持     

Traits of Panax ginseng hairy roots after cold storage and cryopreservation

Summary Panax ginseng hairy root cultures were established by infecting petiole segments with Agrobacterium rhizogenes strain 15834. Hairy root segments including root tips placed onto phytohormone-free 1/2 Murashige and Skoog solid medium and stored at 4 °C in the dark for 4 months, resumed elongation when the temperature was raised to 25 °C in the dark. For cryopreservation, a vitrification method was applied. Root tips precultured with 0.1 mg/l 2,4-D for 3 days and dehydrated with PVS2 solution for 8 minutes prior to immersion into liquid nitrogen had a survival rate of 60 % and could regenerate. The hairy roots regenerated from cryopreserved root tips grew well and showed the same ginsenoside productivity and patterns as those of the control hairy roots cultured continuously at 25 °C. The conservation of T-DNAs in the regenerated hairy roots was proved by PCR analysis.Abbreviations 1/2 MS a half strength Murashige and Skoog (1962) - B5 Gamborg B5 (Gamborg et al. 1968) - WP woody plant (Lloyd and McCown 1980) - RC root culture (Thomas and Davey 1982) - RCI root culture medium containing 100 mg/l myoinositol - HF phytohormone-free - IAA indole-3-acetic acid - IBA indole-3-butyric acid - 2,4-D 2,4-dichlorophenoxyacetic acid - TIBA 2,3,5-triiodobenzoic acid - PCR polymerase chain reaction - PVS2 plant vitrification solution 2 (Sakai et al., 1990) - FDA fluorecein diacetate     

发根农杆菌转化怀地黄再生植株

利用发根农杆菌15834菌株感染怀地黄组培苗子叶、叶柄和茎切段,建立了有效的毛状根培养及其植株再生体系。毛状根可直接从受伤的外植体产生,能在无外源激素的1/2MS固体和液体培养基上自主生长,表现出典型的发根特征。用100μmol/L乙酰丁香酮处理对数生长期的农杆菌菌液感染子叶获得了46.7%的最高转化频率;在附加0.2mg/L KT和3.0mg/L 6/BA的1/2 MS培养基上,毛状根能100%形成愈伤组织,51.49%分化出芽;分化芽在1/2 MS培养基上100%生根,形成具有矮化、节间短和根系发达等特征的转化再生植株且移栽后生长旺盛;1个转化毛状根克隆的梓醇含量为0.557mg/g,是鲜地黄梓醇含量的48.5%,是生地鲜重梓醇含量的18%。rolB基因PCR、Southem blot分析、冠瘿碱纸电泳和RT-PCR扩增检测证明农杆菌Ri质粒上的T-DNA整合到怀地黄基因组中并表达。     

Cryopreservation of Hyoscyamus niger adventitious roots by vitrification

An auxin-independent adventitious root culture of Hyoscyamus niger was established, and the roots were successfully cryopreserved with a high regeneration rate of 93.3 percnt; by vitrification method. The root tips were cultured for 12 to 14 days in phytohormone-free Murashige and Skoog (MS) liquid medium, and were excised and precultured on Woody Plant (WP) solid medium supplemented with 0.3 mol/L sucrose at 25 °C in the dark. After 1 day, they were treated with MS-based loading solution for 10 min, followed by soaking in MS-based PVS2 for 10 min at 0 °C. The treated root tips were immersed in liquid nitrogen (-196 °C). For recovery, the root tips were thawed rapidly at 40 °C and washed with MS medium containing 1 mol/L sucrose prior to plating onto WP solid medium. The regenerated roots were evaluated by their growth and tropane alkaloid production. The growth and alkaloid content of regenerated roots analyzed using HPLC were found to be almost the same as those of non-treated roots.