芥蓝下胚轴离体培养及高频率植株的再生

三个芥蓝品种下胚轴离体植株再生的条件的研究结果表明：下胚轴切口处可直接诱导出芽,诱导“早花尖叶芥蓝”、“中花尖叶芥蓝”和“迟花尖叶芥蓝”直接出芽的最佳激素组合分别为2．0mgL-1BA,0．3mgL-1NAA＋2．0mgL-1BA,0．5mgL-1NAA＋2．0mgL-1BA,其相应的芽发生频率分别为84．6％,86．7％,93．3％。诱导芽发生的最适蔗糖浓度是1％。培养基中加入4．0mgL-1AgNO3和500mgL-1MES可显著提高芽再生频率。再生芽在MS附加0．1mgL-1NAA的培养基上诱导生根形成完整植株。离体再生苗与种子萌发实生苗田间生长外形差别不大,但长势稍慢。     

苦荞胚性愈伤组织诱导与植株再生研究

以苦荞子叶和下胚轴为外植体,进行了不同浓度激素组合的MS和SH固体培养基对胚性愈伤组织诱导及植株再生的研究。结果发现,MS培养基比SH培养基更有利于胚性愈伤组织诱导;2,4-D是诱导愈伤组织的有效激素,KT能有效促进胚状体的形成;下胚轴和子叶都能有效诱导出胚性愈伤组织和再生植株。下胚轴在MS 1.5mg·L-12,4-D 1.5mg·L-1BA培养基,子叶在MS 2mg·L-12,4-D 0.5~1.5mg·L-1BA上能高效诱导出愈伤组织;愈伤组织在MS 2mg·L-12,4-D 0.1mg·L-1KT培养基中继代,能有效诱导胚性愈伤组织;来自下胚轴的胚性愈伤组织在1/2MS 2.0mg·L-1BA 0.5mg·L-1KT 0.1mg·L-1NAA培养基上能够高频再生出芽,来自子叶的胚性愈伤组织在1/2MS 1.0mg·L-1BA 0.1mg·L-1KT 0.1mg·L-1NAA培养基上芽诱导率较高;MS 1mg·L-1NAA是适宜的再生苗生根培养基。     

‘巴斗’杏再生体系的建立与耐盐突变体的筛选

以‘巴斗’杏试管苗茎段为外植体,研究其再生体系的建立以及在含不同浓度NaCl培养基上诱导耐盐愈伤组织,筛选耐盐突变体。结果显示：茎段在MS＋6-BA1．5mg·L^-1＋IBA0．5mg·L^-1培养基上诱导愈伤组织效果最好,芽的分化率可达88％;将出芽愈伤组织块接种到附加IBA0．5mg·L^-1＋KT2．0mg·L^-1的MS分化培养基上效果最佳,芽的分化系数最高为12．7;较理想的生根培养基为MS＋NAA0．1mg·L^-1。＋IBA0．2mg·L^-1,生根率在46．3％以上;在含0．8％NaCl的愈伤组织诱导培养基中,连续继代筛选2代,转入不含NaCl的分化培养基中,分化出了完整植株。经继代培养筛选,测定发现获得的耐盐植株比正常培养植株的游离脯氨酸含量高。     

罗汉果叶片离体再生快繁技术

以罗汉果(Ssiraiti grosvenori)叶片为外植体,探讨培养方式、激素组合对愈伤组织诱导和不定芽分化的影响。结果表明:罗汉果叶片在培养基MS+BA 1.0 mg/L+IBA 0.7 mg/L上培养4周愈伤组织的诱导率达90%以上;罗汉果愈伤组织在培养基MS+BA 1.0 mg/L+IBA0.2 mg/L+赛苯隆(TDZ)0.1 mg/L上不定芽的分化率可达70%,平均出芽指数3.7;罗汉果试管苗在培养基MS+BA 2.0 mg/L+IBA 0.2 mg/L上茎芽增殖比较稳定,在培养基MS+IBA0.1 mg/L上培养2周开始分化不定根,其生根率在90%以上。     

播娘蒿的组织培养和植株再生

TissueCultureandPlantletRegenerationofDescurainiasophiaGAOFu－Li,GAOHong-Bo,LUOPeng,LIAOYan－Hui（InstituteofBotany,SichuanUnionUniversity,Chengdu610064）1植物名称播娘蒿（Descurainiasophia）。2材料类别无菌苗的下胚轴。3培辞条件（1）发芽培养基：MS＋NAA0．1mg·L-1（单位下同）＋6－BA0．1;（2）诱导愈伤组织培养基：MS＋NAA0．2～4．0＋6-BA0．5;（3）诱导分化培养基：MS＋NAA0．2＋6－BA2.0;（4）生根培养基：1／2MS＋NAA0．5或1／2MS＋IBA0.5。上述培养基均加0．7％琼脂、3％蔗糖,pH5…     

牡丹子叶离体再生体系研究

以日本牡丹品种“太阳”为试验材料,研究不同激素组合对牡丹胚初代培养、愈伤组织诱导、分化及植株再生的影响。结果表明：牡丹胚初代培养在1．0mg／L6-BA＋0．25mg／LTDZ的MS培养基上,牡丹胚诱导率最高可达96．1％;剪取无菌子叶转接到附加含有2．0mg／L6-BA＋2．0mg／L2,4-D＋0．2mg／LTDZ的MS培基养上进行愈伤组织培养．诱导率可达100％;愈伤组织在MS＋0．5mg／LKT培养基上分化出芽,分化率达26．6％：不定芽在1／2MS＋1．0mg／LNAA＋4．0mg／LIBA生根培养基上的生根率达27％．     

荞麦组织培养及高频植株再生体系的建立

通过对荞麦(Fagopyrum esculentum Moench)不同外植体、不同激素配比的比较研究,建立了荞麦离体培养高效植株再生体系。荞麦子叶切段在含2．0 mg/L 2,4-D和1．0 mg/L 6-BA的MS培养基上愈伤组织诱导率为89．6％,而下胚轴切段在含2．0 mg/L 2,4-D和1．0-2．0 mg/L 6-BA MS培养基上愈伤组织诱导率高达100％。在2．0 mg／L 6-BA、0．1 mg,L IAA和1 mg／L KT的MS培养基上通过愈伤组织间接分化或外植体直接分化形成不定芽。来自子叶和下胚轴的愈伤组织的分化率分别为42．5％和73．6％,下胚轴的分化率明显高于子叶。将生长状态良好的不定芽转至含1．0 mg/L IBA和0．5mg/L NAA的1/2 MS培养基上生根,生根率达到100％。再生植株移栽到盆土中,成活率达91．6％,并且生长状态和特征均表现正常。     

费尔干猪毛菜愈伤组织的诱导、分化及植株再生体系的建立

探讨了植物生长调节剂、外植体等因子对费尔干猪毛菜（Salsola fergartica Drob．）愈伤组织诱导、分化与植株再生的影响。结果表明：2,4-D与6-BA组合使用时,在一定浓度范围内均有愈伤组织产生,最佳的诱导培养基为MS＋2,4-D2．0mg／L＋6-BA0．2mg／L,下胚轴为诱导愈伤组织的最佳材料;愈伤组织继代培养较好的培养基为MS＋NAA0．1mg／L＋6-BA1．0mg／L;愈伤组织不定芽分化培养基为MS＋6-BA0．5mg／L＋NAA0．05mg／L;根分化的培养基为1／2MS＋IBA0．2mg／L,且生根率可达72％。以带柄子叶为外植体,诱导丛生芽的最佳分化培养基为MS＋6-BA1．0mg／L,再生频率可达90．74％。     

中国木薯栽培种通过器官发生再生植株研究

本文研究了中国木薯栽培种四种外植体通过器官发生再生植株的条件。结果表明:在MS附加0.05mg/L TIBA,1mg/L BA的培养基上“NZ 188”初步的萌发胚状体“切头”后切口处可直接产生丛芽,出芽率为43%。“SC201”胚状体子叶块在MS附加0.5 mg/L NAA,0.5mg/L BA的培养基上可直接出芽,出芽率为42%,在MS附加0.5mg/L IBA,1.5mg/L BA培养基上·出芽率为31%,AgNO_3和ABA单独使用或配合使用均不利于芽的再生。“NZ188”胚状体下胚轴在MS附加0.5mg/LNAA,0.5mg/L BA的培养基上形成的愈伤组织转入MS附加1mg/L NAA,2mg/L BA的培养基上,3周后大多数愈伤组织有绿点出现、仅4.4%外植体分化出芽。“HZ188”无菌苗茎段接种在MS附加0.05mg/L TIBA,2mg/LBA的固体培养基上,2周后形成大量愈伤组织,4周后仅见一块愈伤组织分化出芽。     

油桐叶片愈伤组织诱导及植株再生

以油桐无菌苗叶片为试材,研究不同种类及浓度的植物生长调节剂对愈伤组织诱导、分化、增殖及生根的影响。结果表明：叶片愈伤组织的最佳诱导培养基为1／2MS＋2．omg·L-16-BA＋1．0mg·L～2,4-D,诱导率达100％;最佳分化培养基为1／2MS＋3．0mg·L～6-BA＋0．1mg·L-1。IBA＋0．05mg·L—IAA,分化率为86．36％;最佳继代增殖培养基MS＋3．0mg·L～6-BA＋0．05mg·L。IBA;最佳生根培养基为1／2MS＋O．1mg·L-1。IBA,生根率93．83％。炼苗后移栽到泥炭土：珍珠岩：蛭石=2：1：1的基质中,成活率达92％以上。     

廊坊杨3号快繁和转基因的再生系统

对杂交杨树新品种廊坊杨3号（Populus langfangensis 3,(P. deltoides (“Shan Hai Guan”)×((P. simonii × pyramidalys)₁₂×Ulmus pumila) 的离体叶片和茎段在附加BA、NAA、IBA和2,4-D的MS培养基上的直接和间接的器官分化、愈伤组织形成和植株再生进行了研究。叶柄和叶片最容易在叶脉处直接诱导生芽。从叶片直接诱导生芽的激素条件为1～2 mg·L^-1 BA和0.5 mg·L^-1 IBA,最高生芽率可达90%。2,4-D促进愈伤组织的形成。由愈伤组织诱导生芽的激素条件为0.3～0.5 mg·L^-1 BA 和 0.02 mg·L^-1 IBA或NAA,生芽率达76%。较好的生根条件为0.1 mg·L^-1 BA和0.2～0.5 mg·L^-1 IBA,生根率可达67％。以上再生条件为廊坊杨3号的转基因育种和无性快繁技术提供了可能。     

Efficient procedures for callus induction and adventitious shoot organogenesis in sugar beet (<Emphasis Type="Italic">Beta vulgaris</Emphasis> L.) breeding lines

Summary Improved in vitro tissue culture systems are needed to facilitate the application of transgene technology to the improvement of sugar beet germplasms. Several commercially important sugar beet breeding lines (SDM, 3, 5, 8, 9, 10, 11, HB 526, and CMS 22003) and commercial varieties (Roberta and Gala) were tested for their regeneration capacity through adventitious shoot organogenesis from cotyledons, hypocotyls, root/hypocotyl/shoot transition zone tissues, and leaf lamina and petiole via an intervening callus phase. Callus induction and adventitious shoot regeneration was dependent on genotype and combinations of plant growth regulators. With cotyledon or hypocotyl explants, SDM 3 and 10 showed a better response on adventitious shoot regeneration in medium containing benzyladenine (BA) and 2,3,5-triiodobenzoic acid or 1-naphthaleneacetic acid (NAA) than SDM 11, 5, and 9. Shoot regeneration was obtained from hypocytyl-root or hypocotyl-shoot transition zone tissue in SDM 9, 10, and HB 526 grown on PGo medium supplemented with BA to induce callus, and the regeneration frequency was 25%. Adventitious shoots were also regenerated from leaf explants of SDM 3 and 9 cultured on medium containing NAA for callus induction and BA and NAA to induce shoot regeneration, and in SDM 10 and CSM 22003 cultured on medium containing BA for callus induction and to induce shoot regeneration.     

In vitro culture of Safflower L. cv. Bhima: initiation,growth optimization and organogenesis

Callus induction and in vitro plantlet regeneration systems for safflower (Carthamus tinctorius L.) cv. Bhima using root, hypocotyl, cotyledon and leaf explants were optimized by studying the influence on organogenesis of seedling age, media factors, growth regulators and excision orientation. Supplementation of the medium with an auxin: cytokinin ratio < 1 enhanced the growth rate of callus cultures; however, for 2,4-D the ratio was > 1.34–11.41 μM concentrations of growth regulators (IAA, NAA, BA and Kinetin) in the medium were found effective for callus induction and regeneration in all explants. The calli could be maintained over 32 months. BA (4.43 μM) combined with casein hydrolysate (10 mg l-1) yielded the highest rate of shoot production on hypocotyl (3–6) and cotyledon (5–7) explants and cotyledonary derived callus (4–8). More shoots were produced on explants cut from the most basal region of cotyledons from 5 to 7-day-old seedlings than from older seedlings or more distal cut sites. Apolar placement of explants, inhibited shoot regeneration. The shoot regeneration potential remained upto 7 months in calli developed on NAA + BA. Of three media tested, MS was superior to SH-M and B5. Rooting of shoots was not efficient; 42% of the shoots were rooted on MS medium containing sucrose (7–8%) + IAA (2.8–5.7 μM). Capitula induction was observed in both callus mediated shoots on cotyledons and shoots on rooting medium with sucrose, IAA, NAA and IBA. Well developed plantlets were transferred to the field with a 34% success rate. This revised version was published online in June 2006 with corrections to the Cover Date.     

亚麻组织培养高频不定芽诱导体系

对适合南方地区冬季种植的纤用亚麻品种组织培养过程中基本培养基、激素配比、外植体材料的基因型和苗龄以及再生不定芽的生根条件进行了比较研究。结果表明, 适合于亚麻白花品种组织培养的最佳培养基为YB1, 不定芽诱导率可达98.50%。在此培养基上, 白花、黑亚4号、K6531、K7697、HI026、HI045、I039和阿丽亚那下胚轴不定芽的诱导率分别为98.50%、98.50%、56.50%、42.47%、54.40%、0、27.13%和97.30%, 平均出芽数为11.43、9.33、2.17、0.77、 1.10、0、0.90和10.68。苗龄为7-10天的下胚轴最适于诱导不定芽, 随苗龄增加, 不定芽的诱导率呈下降趋势。RB5培养基最适于不定芽的生根,生根率达100%, 平均生根数为15.3。实验还确定了亚麻对卡那霉素、氨苄青霉素和头孢霉素的抗性浓度阈值。     

亚麻组织培养高频不定芽诱导体系

对适合南方地区冬季种植的纤用亚麻品种组织培养过程中基本培养基、激素配比、外植体材料的基因型和苗龄以及再生不定芽的生根条件进行了比较研究。结果表明,适合于亚麻白花品种组织培养的最佳培养基为YB1,不定芽诱导率可达98.50%。在此培养基上,白花、黑亚4号、K6531、K7697、HI026、HI045、I039和阿丽亚那下胚轴不定芽的诱导率分别为98.50%、98.50%、56.50%、42.47%、54.40%、0、27.13%和97.30%,平均出芽数为11.43、9.33、2.17、0.77、1.10、0、0.90和10.68。苗龄为7-10天的下胚轴最适于诱导不定芽,随苗龄增加,不定芽的诱导率呈下降趋势。RB5培养基最适于不定芽的生根,生根率达100%,平均生根数为15.3。实验还确定了亚麻对卡那霉素、氨苄青霉素和头孢霉素的抗性浓度阈值。     

山茱英的组织培养与植株再生

目的：建立山茱萸的组织培养及植株再生体系。方法：分别以山茱萸的叶片、花柄和花托为材料,进行山茱萸不同外植体的离体培养研究,筛选最佳培养基组成。结果：适宜山茱萸叶片愈伤组织诱导的培养基组合为1／2MS,附加BA2．0mg/L、IBA0,5—1．0mg／L;适宜山茱萸花柄、花托愈伤组织诱导的培养基组合为1／2MS,附加BA1．0mg／L、2,4-D0．5mg／L;在1／2MS附加BA2．0mg／L、IBA0．05mg／L的培养基上,可诱导不定芽的产生;1／2MS附加IBA2．0mg／L的培养基有利于山茱萸试管苗生根。讨论：山茱萸的花托是进行组织培养的最适外植体,白色或翠绿色、结构致密的愈伤组织较易分化产生不定芽。     

广藿香不同外植体离体培养的研究

以广藿香叶片、带节茎、不带节茎及根尖为材料进行离体培养,对影响离体再生的因素进行了研究。结果表明:BA有利于广藿香外植体出芽,浓度以0.1～0.5mg/L效果较好;不同外植体的出芽能力有较大差异,其中以叶片和带节茎出芽能力较强,出芽率均达100%;外植体在培养基上的接种方式对出芽也有一定影响,带节茎以形态学下端垂直插入,可以缩短出芽时间及增加单个外植体出芽的数量。无根苗生根以MT+IBA0.2mg/L培养基为好,苗的生长较为健壮。     

In vitro plantlet regeneration from cotyledons of the tree-legume Leucaena leucocephala

Two plant regeneration methods applicable to Leucaenaleucocephala were developed. In the first method, involvingorganogenesis via callus formation, cotyledon, hypocotyl and root segments wereinitiated on MS medium containing different concentrations ofN⁶-benzyladenine (BA), 2,4-dichlorophenoxyacetic acid (2,4-D), andnaphthaleneacetic acid (NAA). Both compact (type I) and friable (type II) calliwere obtained from the cotyledon and hypocotyl explants treated with differentconcentrations of the growth regulators. Shoots were generated only from thefriable calli formed from the cotyledon explants. The calli formed from thehypocotyl explants did not generate shoots and the root explants died withoutforming callus. Cotyledon explants from 3–4 day old seedlings showedmaximum callus induction compared to those from older seedlings. In a secondmethod involving direct organogenesis, excised cotyledons were cultured on 1/2MS medium containing 10–35 mg l^–1N⁶-benzyladenine (BA) for 7–14 days. Transfer of thecotyledonsto regeneration medium containing low BA resulted in callus formation andsubsequent shoot regeneration from the base of the excised cotyledon explants,with up to 100% frequency. Regenerated shoots rooted best on a basal mediumcontaining no growth regulators.