‘孔府酥脆’枣试管苗离体叶片不定梢诱导和再生

Using in vitro leaves of Zizyphus jujuba ‘Kongfusucui’ plantlet as explants,effects of culture method,phytohormone proportion and culture time on induction rate of adventitious shoot from leaves and effects of sucrose concentrations in rooting media on rooting of adventitious shoot were studied.The results show that induction rate of adventitious shoot by two-step culture method(firstly cultured on medium Ⅰ for four weeks then cultured on medium Ⅱ for three weeks) is significantly higher than that by one-step culture method(cultured continuously on medium Ⅰ for seven weeks).Phytohormone proportion in medium Ⅰ has an obviously influence on induction rate of adventitious shoot,which gradually increases with increasing of TDZ concentration in medium Ⅰ.And adding 1.0 mg·L-1 TDZ in medium Ⅰ leads to induction rate with above 80%.With culture time prolonging(cultured for 1,2,3 or 4 weeks on medium Ⅰ,respectively),induction rate increases gradually.Sucrose concentration has a significant effect on rooting of adventitious shoot,sucrose with higher concentration(30 g·L-1) is beneficial to rooting.According to induction rate and growth status of adventitious shoot,it is determined that optimal culture method of adventitious shoot induction from Z.jujuba ’Kongfusucui’ leaves is two-step culture method,that is,leaves firstly cultured on WPM medium containing 1.0 mg·L-1 TDZ and 0.5 mg·L-1 IAA for four weeks,and then cultured on WPM medium containing 0.5 mg·L-1 IAA and 1.0 mg·L-1 GA3 till adventitious shoot produced.     

‘章姬'草莓茎段愈伤组织诱导及高频植株再生体系的建立北大核心CSCD

In order to cultivate an improved variety with higher potential yield and establish an efficient in vitro regeneration system of strawberry ‘Akihim'(Fragaria × ananassa), callus induction and plant regeneration protocol was designed for solve browning problem. A formal L9(34)orthogonal experiment was designed to investigate the browning research in primary culture using explants of creeping stems excised from aseptic seedlings. Based on the improved medium above, single-factor experiments were conducted to select effective plant growth regulators and appropriate concentrations on blank MS medium. A L9(34)orthogonal experiment was designed to study effects of types and concentrations of plant growth regulators on callus induction, adventitious shoot formation, and plant regeneration. The results indicated that MS medium was inferior to B5 and 1/2MS in inhibiting browning condition. The browning rate was dramatically reduced while the callus still survived on the medium with the addition of 20 g·L-1 Na2S2O3. The callus induction and shoot formation of the explants were observed on MS + 0.1 mg· L-1 6-BA + 0.05 mg·L-1 2, 4-D + 0.1 mg·L-1 NAA with effective inhibiting browning. The optimal medium protocol for multiple shoots proliferation was MS + 0.1 mg·L-1 6-BA + 0.1 mg·L-1 NAA where the proliferation coefficient was 12.86 after 30 d. Healthily regenerated plants were yielded on culture medium 1/2MS + 1.0 g·L-1 AC after 35 d, with a rooting rate of 92.50%. More than 95% of plantlets survived after transplanting into field. The rapid propagation system is helpful to provide homogeneous progeny and high quality seedlings for cultivation of strawberry ‘Akihime' as well as a technical reference for other strawberry species in vitro regeneration. [ABSTRACT FROM AUTHOR]     

In vitro plant regeneration of Aristolochia indica through axillary shoot multiplication and organogenesis

Protocols for in vitro plant regeneration via axillary and adventitious shoot regeneration were established in an important medicinal plant, Aristolochia indica L. (Aristolochiaceae). Basal Murashige and Skoog's (MS) medium supplemented with 0.54 μM α-naphthaleneacetic acid (NAA) and 13.31 μM benzyladenine (BA) induced the maximum number of shoots (45-50) from shoot tip and nodal segment cultures. Phenolic accumulation in leaf and internodal stem derived callus cultured in MS medium containing NAA or 2,4-dichlorophenoxyacetic acid and BA or kinetin was controlled by the addition of 1.0 mg l^-1 phloroglucinol (PG) to the callus induction medium. Basal medium supplemented with 2.69 μM NAA, 13.31 μM BA and 1.0 mg l^-1 PG induced the best results in terms of shoot bud regeneration from leaf derived callus. Direct de novo development of shoots from leaf segments was achieved using 13.31 μM BA along with 50 mg l^-1 activated charcoal. The microshoots were rooted in White's medium supplemented with 2.46 μM indolebutyric acid. More than 85% of rooted plants survived in the soil. This revised version was published online in June 2006 with corrections to the Cover Date.     

'红香芋'茎尖玻璃化法保存条件的筛选

In order to screen suitable vitrification conservation conditions for shoot tip of Colocasia esculenta'Hongxiangyu', pre?culture, vitrification protection and thawing conditions were compared. The results show that with increasing of sucrose concentration in the medium and extending of pre?culture time, survival rate of shoot tip increases gradually. After different loaded and dehydrated measures, water content in shoot tip is lower than that of the control, while survival rate of shoot tip increases significantly than that of the control. Thawing for 1-2 min at 40℃-60℃ generally has no significant effect on survival rate of shoot tip. Suitable cryopreservation steps of vitrification as follows: shoot tip pre?cultured for 3 d in medium with 06 mol·L-1 sucrose firstly, then loaded for 30 min in 60% PVS2, dehydrated for 15 min in PVS2, put in PVS2 and conserved in liquid nitrogen, and shoot tip thawed for 1-2 min in 40 ℃.     

Genetic transformation of gentian using wild-type Agrobacterium rhizogenes

Leaf sections of greenhouse-grown Miscanthus x ogiformis Honda 'Giganteus' plants and leaf sections or shoot apices of in vitro shoot cultures were grown on Murashige and Skoog medium containing various concentrations of benzyladenine (BA) and 2,4-dichlorophenoxyacetic acid. On leaf sections, the callus induction decreased with increasing BA concentration. The percentage of embryogenic callus was increased, the percentage of root-forming callus decreased, and a new shoot-forming callus type was formed by inclusion of BA during callus induction. A higher percentage of shoot-forming callus was formed on shoot apices compared with leaf sections of in vitro-grown shoots when cultured on 0.4 μM BA. The largest number of plants per callus piece was regenerated from shoot-forming callus, but maintenance of the high regeneration capacity proved difficult. This revised version was published online in June 2006 with corrections to the Cover Date.     

Anther culture and haploid plant regeneration in purple coneflower (Echinacea purpurea L.)

Anthers containing microspores at the uninucleate stage were excised from capitula of field grown plants of purple coneflower, Echinacea purpurea, and cultured on medium conducive to callus growth. In callus induction cultures, N6 basal medium was more effective than Murashige and Skoog (MS), and a combination of benzyladenine (BA) at 2.22 μM with naphthaleneacetic acid (NAA) at 0.054 μM was more effective than 2,4-dichlorophenoxyacetic acid (2,4-D) alone at 4.52, 9.05 and 13.57 μM. Callus induction rate as high as 85.8% was achieved, and no statistically significant differences were found among cultures with various densities of 20, 40, 60, 80 and 100 anthers per bottle each filled with 40-ml medium. Shoots were regenerated from calluses on MS medium containing 2.22 μM BA and various concentrations of NAA, with the highest regeneration rate of 95.24% obtained when 0.27 μM NAA was applied. Although a large portion of the␣regenerated shoots had prominent symptom of vitrification, some normal shoots could be easily rooted on MS medium containing 0.054 μM NAA. Thirty regenerated plants were randomly selected and 19 of them were confirmed to be haploid by observation of chromosome number of root-tip cells.     

芫花的花粉形态观察及生活力和萌发率分析

Pollen morphology of Daphne genkwa Sieb.et Zucc.was observed by scanning electron microscope(SEM),and its viability and germination rate were measured by TTC and sucrose in vitro culture methods.The results show that pollen is stenopalynous type with a diameter of 15.6-21.6 μm.Per pollen has 10-16 apertures which is irregular circular with a diameter of 1.4-2.0 μm.Surface ornamentation of pollen is rough reticulate pattern which is circular polygon(tetragon-heptagon,mostly pentagon-hexagon).Pollen viability is 51% by TTC.Sucrose of different concentrations has a significant effect on pollen germination rate during pollen culture.And pollen germination rate is the highest with a percentage of 27.0% in medium containing 50 g·L-1 sucrose,while pollen could not germinate in medium containing sucrose over 250 g·L-1.Otherwise,there is the phenomenon of "multi-aperture germination" during pollen germinating.     

Embryogenic callus formation,growth and regeneration in callus and suspension cultures of Miscanthus x ogiformis Honda Giganteus' as affected by proline

The effects of proline additions to culture systems of Miscanthus x ogiformis Honda Giganteus' were investigated. Proline was added in concentrations of 0, 12.5, 25, 50, 100 or 300 mM to the callus induction and suspension culture media containing either Murashige and Skoog or N6 basal salts and 22.6 μM 2,4-dichlorophenoxyacetic acid. Shoot apices and leaves from in vitro-propagated shoots, and immature inflorescences from greenhouse-grown plants were used as explants for callus induction and formation. Suspension cultures initiated from embryogenic callus of immature inflorescences were used to test the effect of proline in suspension cultures. The proline additions affected the formation of embryogenic callus and the growth of suspension cultures. Improvements depended on the proline concentration and the basal salts of the medium. Addition of 12.5 to 50 mM proline to callus induction medium with Murashige and Skoog salts increased embryogenic callus formation on shoot apices and leaf explants while proline had no effect on embryogenic callus formation in medium with N6 salts. Increased growth with increasing proline concentration was obtained in suspension aggregates grown in medium with N6 salts, whereas proline only increased growth of suspension aggregates grown in medium with Murashige and Skoog salts at concentrations of 12.5 or 25 mM. A stimulating effect of proline on plant regeneration was observed in short-term cultures of callus as well as in long-term cultures of suspension aggregates. An optimum proline concentration for plant regeneration was found at 12.5 mM. This revised version was published online in June 2006 with corrections to the Cover Date.     

High auxin stimulates callus through SDG8-mediated histone H3K36 methylation in Arabidopsis

Callus induction,which results in fate transition in plant cells,is considered as the first and key step for plant regeneration.This process can be stimulated in different tissues by a callus-inducing medium(CIM),which contains a high concentration of phytohormone auxin.Although a few key regulators for callus induction have been identified,the multiple aspects of the regulatory mechanism driven by high levels of auxin still need further investigation.Here,we find that high auxin induces callus ...     

Effects of medium components and light on callus induction, growth, and frond regeneration in Lemna gibba (Duckweed)

Summary Basal media, plant growth regulator type and concentration, sucrose, and light were examined for their effects on duckweed (Lemna gibba) frond proliferation, callus induction and growth, and frond regeneration. Murashige and Skoog medium proved best for callus induction and growth, while Schenk and Hildebrandt medium proved best for frond proliferation. The ability of auxin to induce callus was associated with the relative strength of the four auxins tested, with 20 or 50 μM 2,4-dichlorophenoxyacetic acid giving the highest frequency (10%) of fronds producing callus. Auxin combinations did not improve callus induction frequency. Auxin in combination with other plant growth regulators was needed for long-term callus growth; the two superior plant growth regulator combinations were 10 μM naphthaleneacetic acid, 10 μM gibberellic acid, and 2 μM benzyladenine with either 1 or 20 μM 2,4-dichlorophenoxyacetic acid. Three percent sucrose was best for callus induction and growth. Callus induction and growth required light. Callus that proliferated from each frond’s meristematic zone contained a mixture of dedifferentiated and somewhat organized cell masses. Continual callus selection was required to produce mostly dedifferentiated, slow-growing callus cell lines. Frond regeneration occurred on Schenk and Hildebrandt medium without plant growth regulators but was promoted by 1 μM benzyladenine. Callus maintained its ability to regenerate fronds for at least 10 mo. Regenerated fronds showed a slower growth rate than normal fronds and a low percentage of abnormal morphologies that reverted to normal after one or two subcultures.     

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。     

影响四季桔器官发生的因素

对四季桔胚轴直接出芽、愈伤组织诱导及植株再生能力的研究表明：上、下胚轴在含有BA的MT培养基上,均能直接出芽,但上胚轴出芽能力明显高于下胚轴,最高出芽率为96．9％。外植体在培养基上的接种方式,对出芽也有一定影响,上胚轴切段以形态学下端垂直插入,出芽率高,且在培养前期表现尤为突出。胚轴愈伤诱导的适宜培养基为MT＋IBA0．5mg-1＋BAgmg-1。愈伤组织分化时,上、下胚轴愈伤组织所要求的BA浓度分别为4mgL-1及2mgL-1。在根的诱导中,附加的生长素种类,不仅影响生根率的高低,而且影响上部茎叶的生长,其中以加入lmgL-1IBA的效果最好,生根率达84．4％。     

多花黄精诱导愈伤组织与不定芽培养基筛选

以多花黄精Polygonatum cyrtonema的根状茎为外植体,通过L9(34)正交试验比较不同植物生长调节剂及其组合对多花黄精愈伤组织诱导的影响,筛选最适生长调节剂配方,同时筛选通过器官发生方式直接成芽较为合适的培养基。结果表明,含有2,4-D和KT的培养基诱导愈伤组织效果显著,多花黄精愈伤组织诱导的最适培养基为MS + 6-BA 2.0 mg·L-1 + 2,4-D 0.5 mg·L-1 + NAA 0.1 mg·L-1 + KT 1.0 mg·L-1,该培养基的愈伤组织诱导率可达39.10%;培养基MS + 6-BA 4.0 mg·L-1 + NAA 0.2 mg·L-1可诱导多花黄精根状茎直接产生不定芽。     

红籽鸢尾高频离体再生条件的初步筛选

红籽鸢尾(Iris foetidissima Linn.)为鸢尾科(Iridaceae)鸢尾属(Iris Linn.)多年生草本植物,原产于西欧和非洲北部。该种的叶鞘呈深绿色剑形,蒴果饱满且蒴果成熟开裂后露出红、橙黄和白等不同色泽的种子并一直垂挂到翌年春天,集观花、观叶和观果为一体,观赏价值较高。另外,该种还具有耐寒性好、在长江中下游地区四季常绿、适应性强及耐粗放管理等优     

药用植物栀子的组织培养

栀子(Gardenia jasminoides)为药用木本植物。以栀子果皮、种子团和种子为外植体,研究不同激素配比及不同培养方式对愈伤组织诱导和芽分化的影响。研究结果表明,培养基成分为MS+0.5 mg·L–12,4-D+0.25 mg·L–16-BA较适宜果皮和种子愈伤组织的诱导,诱导率分别为83.3%和88.5%;培养基成分为MS+1.0 mg·L–12,4-D+1.0 mg·L–16-BA较适宜种子团愈伤组织的诱导,诱导率为78.1%。3种外植体诱导的愈伤组织中,只有种子愈伤组织能通过液体培养分化出芽;TDZ对芽分化有明显的促进作用;最佳的芽分化培养基为MS+0.05 mg·L–1NAA+0.10 mg·L–1TDZ,其愈伤组织分化率为8.75%。该研究以栀子种子为外植体,并获得了再生植株,为药用植物栀子转基因体系的建立奠定了基础。     

菘蓝花药培养及单倍体的诱导

探讨菘蓝花药处于单核晚期的形态指标,并以适宜发育时期的花药为外植体,进行花药培养及单倍体诱导。实验结果表明,4℃低温处理2d后,在含有6-BA0．5mg·L-1和NAA1．0mg·L-1。的Ms培养基上,花药愈伤组织的诱导率为23．35％;将其转接到Ms附加6．BA1．0mg·L-1,NAA0．5mg·L-1的分化培养基上,80．00％以上的愈伤组织可以诱导产生不定芽;再将分化出的试管苗转接到1／2MS＋NAA1．0mg·L-1的生根培养基上,3d左右即可获得完整植株。经叶边缘压片检查染色体数目,花药培养所得的弱小绿苗为单倍体植株。     

火龙果愈伤组织诱导与植株再生

为了建立火龙果愈伤组织诱导与植株再生体系,以火龙果茎段、幼苗和子叶为外植体进行离体培养试验。结果表明：茎段诱导愈伤组织的最优培养基为1／2MS＋2,4-D2．0mg·L^-1＋6-BAO．5mg·L^-1,诱导子叶愈伤组织的最适培养基是1／2MS＋2,4-D2．0mg·L^-1＋6-BA1．0mg·L^-1,诱导愈伤组织分化的最优培养基为1／2MS＋6-BA4．0mg·L^-1＋NAA0．5mg·L^-1,最佳生根培养基为1／2MS＋6．BA1mg·L^-1＋NAA0-3mg·L^-1。     

甜叶菊茎段腋芽诱导培养基和NaN3诱变条件筛选及诱变试管苗POD同工酶分析

以甜叶菊(Stevia rebaudiana Bertoni)茎段为外植体,采用L9(34)正交表对腋芽诱导培养基中的激素种类和浓度(0.0、0.1和0.2 ng·L-1NAA;0.0、0.5和1.0 mg·L-16-BA;0.000、0.005和0.010 mg·L-1TDZ)进行筛选;在此基础上对诱变过程中NaN3溶液的浓度(3、6和9 mmol·L-1)和处理时间(1、2、4和8h)进行比较,并初步筛选出最佳的NaN3诱变条件;采用聚丙烯酰胺凝胶电泳法(PAGE)对经上述NaN3诱变处理后培养5、10和15 d的试管苗POD同工酶酶谱的变化进行了分析.结果表明:在添加了不同激素组合的培养基上均能诱导出腋芽,但腋芽数和苗高有差异;经综合比较后可确定适宜于甜叶菊腋芽诱导的培养基为添加1.0 mg·L-16-BA和0.1 mg·L-1NAA的MS培养基(含5.0g·L-1琼脂粉和30g·L-1蔗糖,pH 6.0).经NaN3诱变处理后,茎段在腋芽诱导培养过程中的死亡率随NaN3浓度提高和处理时间延长逐渐增加,平均腋芽数和苗高则下降,且多数处理组试管苗矮化;根据半致死剂量确定的最佳NaN3诱变处理方法为将甜叶菊茎段置于9 mmol·L-1 NaN3溶液中浸泡4h.PAGE分析结果表明:甜叶菊诱变试管苗的POD同工酶谱均可分为a、b和c区,但在不同培养时间各处理组POD同工酶的条带数和活性有所变化.在培养5和10 d后各处理组诱变试管苗POD同工酶的活性和条带数量有明显差异,而在培养15 d后各处理组诱变试管苗POD同工酶活性有差异,但条带数量没有明显变化,表明用适宜浓度的NaN3进行诱变处理可导致甜叶菊试管苗短期的应激效应.     

不同激素对银斑百里香愈伤组织培养的影响

以银斑百里香种子为试材,比较了不同浓度的NAA和2,4-D与6-BA对百里香愈伤组织诱导效果的影响。结果表明:NAA在0.15(mg/L)和2,4-D在0.9(mg/L)是诱导银斑百里香种子产生愈伤组织的最佳浓度;MS+NAA(0.15mg/L)+6-BA(0.6mg/L)和MS+2,4-D(0.9mg/L)+6-BA(0.6mg/L)诱导的效果最佳,建立了百里香愈伤组织培养的实验体系。     

细裂银叶菊叶的组织培养繁殖研究

以细裂银叶菊叶片为材料,进行愈伤组织的诱导、分化培养及生根诱导培养。结果表明：叶片愈伤组织的诱导以MS 2,4-D2mgL^-1 BA1mgL^-1 NAA0．1mgL^-1。培养基较好：分化培养以MStBA0．5mgL^-1 NAA0．1mgL^-1为好：生根诱导以1／2MS NAA0．01mgL^-4效果最好。