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1.
表油菜素内酯对拟南芥细胞分化的影响 总被引:6,自引:0,他引:6
研究了表油菜素内酯对拟南芥细胞体外分泌的影响,表明epi-BR不仅能促进愈伤组织的增殖,而且还能有效地诱导愈伤组织转绿,继而分化绿芽长成小植株,其诱导频率高达70%以上,电镜观察表明,epi-BR诱导的转绿细胞中的叶绿体发育正常。 相似文献
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外源激素对金钱松胚外植体愈伤组织的诱导及其器官发生的调节作用 总被引:5,自引:0,他引:5
金钱松胚外植体在培养过程中由于外源激素的种类和配比的不同而存在着几种发育途径:直接从胚外植体表面分化不定芽;先诱导愈伤组织,再从愈伤组织分化不定芽;还可由愈伤组织分化出胚状体。激素BA对外植体不定芽的诱导起着关键作用。激素2,4-D则诱导愈伤组织,BA与2,4-D配比恰当诱导的愈伤组织分化出体细胞胚状体。 LP’附加低浓度的BA或KT(<0.5mg/L)促进不定芽茎的伸长; LP’附加浓度的IBA(<0.5mg/L)诱导不定根的发生。愈伤组织在基本培养基浓度为 ×LP’或1×LP’的分化培养基上不定芽诱导率相似。 相似文献
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ABA,NAA诱导水稻胚性愈伤组织的研究 总被引:14,自引:0,他引:14
ABA和NAA联合使用能有效地诱导水稻原生质体再生的愈伤组织向胚性发展。通过液体浅层培养由原生质体得到的愈伤性发展。通过液体浅层培养由原生质体得到的愈伤组织,在含ABA和NAA的N8培养基上培养一段时间,可以诱导原来呈非胚性状态的愈伤组织形成胚性愈伤组织,并在含ZT的N6分化培养基上产生绿点。通过对这两种愈伤组织的生化分析,表明二者在游离氨基酸、DNA、RNA、核酸及蛋白质含量等方面,特别是SDS 相似文献
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表油菜素内酯对黄瓜子叶过氧化物酶活性和可溶性蛋白含量的影响 总被引:3,自引:0,他引:3
0.5mg/L的表油菜素内酯(epi-BR)能显著地促进黄瓜子叶叶绿素a、叶绿素b的含量和叶绿素a/叶绿素b比值的下降,表明eni-BR能促进子叶的衰老。从过氧化物酶(POD)的活性测定及同工酶谱发现epi-BR可提高其活性,暗示它可能通过提高子叶POD的活性而加速子叶叶绿素的降解。另一方面,epi-BR促进子时可溶性蛋白含量的下降,其中主要是RuBP羧化酶含量的下降,同时,epi-BR引起子叶游离氨基酸的累积。 相似文献
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水稻花药液体培养下影响愈伤组织诱导和分化的一些因素的研究 总被引:3,自引:0,他引:3
水稻花药液体漂浮培养能大幅度提高愈伤组织诱导频率,但这些愈伤组织的分化能力很低。为了提高液体培养下愈伤组织的分化频率,试验了5种诱导培养基和4种分化培养基。结果表明,诱导培养基对愈伤组织分化能力的高低起主要作用,其中以过滤灭菌的马铃薯提取液培养基的效果最好,绿苗分化率可高达50%;分化培养基对愈伤组织分化频率的影响较小,且不甚规律。浮在液面上的愈伤组织比沉在培养液底部的愈伤组织有较高的分化能力。愈伤组织转移时间的早晚对分化频率也有很大影响。 相似文献
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《Acta Botanica Sinica》1975,(4)
3年来通过对籼稻(Oryza sativa subsp.hsien)花药培养的研究,愈伤组织的诱导率从0.2%提高到平均为2.85%,最高达18.75%;绿苗分化率从5%以下提高到平均为13.1%最高达到45.5%。在6个籼稻品种、38个籼×籼杂种中成功地诱导出了绿苗。本文着重研究了提高诱导率的有关因素。以单核晚期花粉的花药愈伤组织诱导频率最高。籼稻花粉去分化过程相对地要求较低浓度的培养基,籼稻花药对高浓度的改良 RM-1964培养基完全没反应。用杂种的诱导率较亲本材料为高。以易于诱导愈伤组织或易于分化绿苗的品种作亲本的杂种后代,诱导率与绿苗分化率亦较高。籼稻形成愈伤组织的高峰是在接种后的50—60天之间。愈伤组织分化的高潮是在转移后10—30天之间。籼稻愈伤组织的分化以先分化根的类型最多,在先分化根的愈伤组织中有36.74%能再分化出芽来。 相似文献
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影响小麦花粉植株分化的几个因素 总被引:1,自引:0,他引:1
以小麦杂种F1代花粉愈伤组织为材料,研究了影响花粉植株分化的几个因素。试验结果表明,随着花药培养时间的延长.其愈伤组织的分化能力逐渐降低;分化培养基中附加KT和BA两种细胞分裂素相结合有利于绿苗分化;4℃─5℃低温处理愈伤组织24小时能提高绿苗分化率。 相似文献
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提高小麦愈伤组织分化频率的因素 总被引:52,自引:0,他引:52
研究了影响小麦愈伤组织诱导、芽分化及其植株再生的一些因素。结果表明:在愈伤组织诱导和继代过程中添加ABA(1.0mg/L)有利于小麦中晚期幼胚致密愈伤组织的诱导及再生能力的保持;外植体来源尤其是基因型对长期培养的愈伤组织再生能力有很大影响;不同的外源激素(KT、6-BA、IAA、TDZ和玉米素等)也影响芽分化频率,其中TDZ可明显提高芽分化频率;在转入分化培养前对愈伤组织进行干燥处理可有效地提高其 相似文献
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发根土壤杆菌Ri质粒对黄瓜进行遗传转化的研究 总被引:3,自引:1,他引:3
以发根土壤杆菌Ri质粒介导,对载体pBTC-8上的T-DNA转化黄瓜进行了初步研究。采用黄瓜的各种不同外植体片断与土壤直菌共培养的方法,诱导出具有典型毛状根特性的转化根,转化根经诱导培养形成愈伤组织,冠瘿碱检测表明,转化根及愈伤组织含有农杆碱和甘露碱。愈伤组织进一步分化培养再生出完整植株。再生植株表现卡那霉素抗性。 相似文献
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自1979年Grove等首次从油菜(&.wM-。。WL·)花粉中分离出油菜素内酯(brassinolide,BR)以来,人们已在该激素的生理反应和对植物生长发育等方面进行了许多研究(Kalinich等1985,Mandava1988,吴登如和赵硫橘1993)。但由于这类激素在10-'mol/L浓度水平就能诱导大豆、水稻等多种植物细胞的生长和分裂(Sasse1991),而且在植物体内含量极低,因此用传统的方法研究它的作用方式非常困难。目前,利用激素突变体来研究激素代谢及其分子机制已有不少成功的例子,如生长素(Keily和Bradford1986,Lincoln等1990)、赤霉素(Singh… 相似文献
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本研究以羊草(L eym us ch inensis)与灰色赖草(L eym us cinereus)杂种F1代幼穗为外植体诱导愈伤组织,在3.0 m g/L 2,4-D M S培养基上继代1次后,转入不同浓度激素(2,4-D、IAA、KT)配比和不同浓度蔗糖的M S液体培养基进行振荡培养,建立杂种F1代细胞悬浮系和植株再生体系.结果表明,细胞悬浮培养时,M S 1.0 m g/L2,4-D 0.1 m g/L KT 4%蔗糖的液体培养基最佳;悬浮细胞分化时,1.0 m g/L 2,4-D 0.1 m g/L KT 4%蔗糖 M S和1.0 m g/L 2,4-D 4%蔗糖 M S培养的悬浮细胞在1.0 m g/L NAA 0.5 m g/L KT M S分化培养基上的绿苗分化率分别达到83%和80%.细胞悬浮系及再生体系的建立为杂种F1代育性恢复的研究奠定了基础. 相似文献
14.
paper deals with regeneration of protoplasts in cell suspension cultures of hypocothl from Trifolium lupinaster L. on the SL2 basal medium with BA 0.1 mg/L and picloram 0.06 mg/L for 3--4 month,s. The protopiasts were isolated from suspensions cells subcultured for 3 days and were recuhured in modified liguid medium 8p. The first division of the regenerated cell occurred 3 days after being cultured in medium Bp. Small calli could be seen with naked eyes by one month. The calli when grew up to 2 mm long, were transferred in succession differentiation medium A and B for organ differentiation. The differentiated shoots formed their roots on 1/2 MS supplamented with NAA 1.0mg/L and then grew into plantlets. 相似文献
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火炬松成熟合子胚培养直接器官发生和植株再生 总被引:11,自引:0,他引:11
基因型Hb,Ma和Mc的火炬松成熟合子胚在附加1.0mg/LNAA,4.0mg/LBA,500mg/LLH和500mg/L谷氨酰胺的TE培养基上培养12周后,在子叶和胚轴部位形成不定芽原基。然后将合子胚转移到附加0.5mg//LNAA,0.05mg/LIBA,2mg/LBA,500mg/LLH和500mg/L谷氨酰胺的TE不定芽分化培养基上,6周后分化产生大量不定芽,3种基因型中,Hb的直接不定芽 相似文献
16.
Calli produced from stem segments of seedling of Coriandrum satwum which were cultured on MS agar medium containing NAA 1.0mg/L. The embryogenic cell colony suspension was estabilished on MS liquid medium containing NAA 1.0mg/L%2,4-D 0.2mg/L+BA 0.5 mg/L. The cell suspension culture was used for protoplast preparation. Protoplasts were obtained in the enzyme mixture containing 2.0% Onozuka R-10, 1.0% pectinase, 0.5% snailase, 0.5% dextran sulfate potassium Salt, 0.6mol/L mannital CPW solution at pH 5.8 and 25℃. Cultured in a KM8P liquid medium containing NAA 1.0mg/L+2,4-D 0.2mg/L+6-BA 0.5 mg/L, glucose 0.4mol/L and CM 20mi/L; the protoplasts entered the stage of derision after three days, cell clusters formed in 10 days and calli formed after about 50 days. When the calli were transferred to MS agar medium containing many growth substances, they differentiated into embryoids, and then developed into plantlet with many green leaves and roots on the 1/2 MS agar medium. 相似文献
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墨兰的无菌播种结果发现,在不添加细胞分裂素的培养基上,种子可以发芽,但只有原球茎和根状茎产生;不可能进一步分化成苗,只有在含有不同激素成分的MS或KnudsonC培养基上,才有可能诱导芽的分化,其中以附加6-BA 0.5-1.0mg/L+NAA 0.1mg/L诱导效果最佳,在附加6-BA 2.0mg/L+NAA 0.4mg/L的MS培养基中,能加速芽的增殖,根状茎转入含有相同激素成分的液体增殖培养基中振荡培养,可大大提高芽的分化速率。添加0.5%活性炭对芽的分化有明显增效作用。在附加NAA 0.2mg/L的MS培养基中;幼苗的生根效果最佳。 相似文献
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Protoplasts isolated from 3--4 day-old (ca 4 cm in length) etiolated hypocotyls of Brassica carnpestris var. parachinesis (Bally) Tsen et Lee and purified with 20% sucrose were cultured on K8p medium suplemented with 0. 5 mg/L ZT, 0.5 mg/L 2, 4-D, 1.0 mg/L NAA and 0. 4 mol/L glucose. When initially cultured for 14-18 hours the protoplasts formed new walls and by first division after 36 hours. The divided protoplasts reached 35 % after being cultured for three days. When cultured under optimum conditions for 8-9 days, the proto plasts formed 8-16 cell colonies with a plate effeciency as high as 15%-18%. Rapidly growing and dividing calli of 2 mm in diameter were transferred onto semisold gelrite media with 0.3 mg/L 2, 4-D enabling them to proliferate further towards the size of 4-5 mm in diameter. Shoot differentiation was carried out in MS medium with 3.2 (or 1.6) mg/L BA, 1.6 (or 0.8) mg/L ZT, 0.01 mg/L NAA, 0. 1 mg/L GA3 and 0.2 % sucrose. Shoots were cut down and rooted on medium with 0.2 mg/L IAA and 2 % sucrose where whole plants were evatually developed. 相似文献
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Daxu Li Jie Zhang Jian Zhao Yi Zhang Fei Chen Jingqiu Zhu Shujun Liu Zhirong Yang 《Plant Cell, Tissue and Organ Culture》2006,84(3):285-292
The mature seeds, mesocotyls, and young leaf tips of Elymus sibiricus L. cv. ‘chuancao No. 2’ were cultured on Murashige and Skoog (MS) medium supplemented with 5.0 mg/L 2,4-dichlorophenoxyacetic acid (2,4-d) and 0.05 mg/L kinetin in the dark at 26°C, the calluses were produced. The rate of callus regeneration depended on the explants
source and plant growth regulators. Plants regenerated from whitish-yellow-coloured compact nodular callus formed after subculturing
for 8 weeks. Higher frequency (54%) of shoot differentiation was obtained from the embryo tissues of mature seed than from
either mesocotyls (24%) or young leaf tip tissues (6%) when these calluses from different types of explants were cultured
on plant regeneration medium containing half strength MS salts supplemented with 0.1 mg/L kinetin, 1.5 mg/L 2,4-D and 20 g/L sucrose. The green plants were rooted within 6 weeks in the root regeneration medium, and over 97% of these soil-established
plants were obtained in the greenhouse when potted in a sand and peat mixture medium. 相似文献
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由枸杞髓部组织诱导出胚性愈伤组织,并由此愈伤组织建立起稳定的细胞悬浮系。从悬浮细胞游离的原生质体在改良KM培养基(1.5 mg/L 6_BA,0.5 mg/L NAA和0.5 mg/L 2,4_D)中进行液体浅层培养,3~4 d后出现第一次分裂,第7 d统计分裂频率为50.3%,15 d左右可形成细胞团,3~4周后形成肉眼可见的愈伤组织,愈伤组织植板率为1.25%。将细胞团转移到液体分化培养基(MS+6_BA 1.5 mg/L+2,4_D 0.2 mg/L) 8~10 d可形成大量胚状体,及时将胚性愈伤组织块转移到固体分化培养基上(MS+6_BA 0.2 mg/L),可形成大量绿芽,分化率54.17%。绿芽在生根培养基(MS+NAA 0.2 mg/L)可形成完整植株,移栽后成活良好。 相似文献