棉胚珠愈伤组织诱导纤维分化初探（简报）

开花当天的棉花胚珠切块在MS－GA3培养基上愈伤组织快速形成，随着时间年龄的增加，过氧化物酶活性变化平缓，纤维诱导分化率高；而在MS－2，4－D培养基上，愈伤组织生长缓慢，过氧化物酶活性起伏上升，整个过程中纤维诱导分化率差别不大。     

骆驼蓬的组织培养及植株再生

以骆驼蓬(Peganum harmala L)无菌苗下胚轴切段为材料,在不同的培养基上进行愈伤组织的诱导,发现在MS基本培养基附加2．0mg/L 2,4—D、0．5mg／L 6—BA和3％蔗糖时,可100％的诱导出愈伤组织。愈伤组织在附加2．0mg／L 6—BA、0．5mg／L NAA、500mg／L CH和3％蔗糖的MS培养基上诱导出丛生芽,进而发育成苗,苗的分化频率在30％左右。分化苗或其茎切断在附加0．2mg／L IBA、0．2mg/L NAA和3％蔗糖的l／2MS培养基上出现根的分化,分化频率在90％以上。再生植株经炼苗后移栽成活,成活率在80％以上。     

甘薯叶片组织培养一次成苗的研究

以甘薯叶片为外植体,在附加有不同植物激素的MS培养基上均诱导出愈伤组织,其中附加0.16mg/LNAA和1.0mg/LBA的MS培养基是诱导愈伤组织的适宜培养基。芽的分化在处理、基因型间差异较大,其中诱导芽分化的最佳培养基为附加1.0mg/LNAA、0.1mg/LBA和0.1mg/LABA的MS培养基。在所试的3个品种中,济南红分化率最高,宁-331次之,千系-682最差。最高分化率为21.5%,是前人报道最高分化率（11.0%）的1.95倍。分化苗移栽成活率达100%,大多数保持了原品种的特性。本文对生长素、细胞分裂素、ABA对器官分化的影响做了讨论。     

墨兰的无菌播种和植株再生

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。     

沙葱(Allium mongolicum Regel)离体培养再生可育植株

以沙葱（Allium mongolicum Regel)的叶基切段作外植体,成功地诱导出愈伤组织和再生植株。诱导愈僵组织的培养基为附加2mgL^-22,4-D和0.2mgL^-1KT的MS培养基。愈伤组织转移到附加2mgL^-16BA和0.4mgL^-1NAA的MS培养基后分化出大量的苗;分化苗在含有IBA1mgL^-1的1/2MS培养基上生根最佳。再生植株移栽成活率在95%以上。移栽到田间的植株第二年以后可正常开花结实。     

马铃薯未传粉子房离体培养诱导双单倍体植株

以MS为基本培养基,附加不同水平的生长素,培养未传粉马铃薯子房,经三年试验,从两个品种中获得了双单倍体的绿色小植株,(2n=2x=24);从分化绿苗力很强的球状愈伤组织中,又不断地分化出许多绿色小植株。绝大多数品种,都可以诱导出愈伤组织,一般诱导率为70％左右。品种的基因型和培养基中的生长素种类与水平在愈伤组织分化绿苗中起着重要作用。通过扦插和试管微型薯培养,可以大量繁殖试管苗,这为马铃薯单倍体育种提供了较有利的条件。     

地黄组织培养及植株再生的研究

以地黄根茎所获无菌苗为材料,对其愈伤组织诱导、分化和再生植株的获取进行了初步研究。结果表明：取叶片、茎段、叶柄进行愈伤组织诱导,筛选出最适培养基为MS附加2,4-D0．5mg／L、BA1．0mg／L,愈伤组织诱导率可达100％。将叶片接种在分化培养基中,诱导不定芽,其最适分化培养基为MS附加BA 3mg／L、NAA 0．1mg／L,分化率为77．5％。试管苗在改良的MS(大量与微量元素、铁盐和有机物质各1／2)附加NAA 0．05mg／L的培养基上,经过15～20d培养,生根率可达100％。     

大叶秦艽的组织培养与植株再生

以秦艽的叶和下胚轴为外植体,成功地诱导出愈伤组织和再生植株.诱导愈伤组织最合适的培养基为附加2 m g·L- 1 2 ,4 - D和0 .5 mg·L- 1 6 - BA的MS培养基,诱导率可达到10 0 % .愈伤组织转移到附加2 mg·L- 12 ,4 - D和0 .5 mg·L- 1 KT和5 0 0 m g·L- 1 L H的MS培养基上进行继代培养,增殖后的愈伤组织转移到附加0 .1mg·L- 1 2 ,4 - D和0 .5 m g·L- 1 6 - BA的MS分化培养基上进行分化,其分化率可达到86 .6 7% ,将分化出的芽转接到不加激素的MS上,结果可生长出大量的分化苗.     

小麦胚乳愈伤组织的诱导及分化的研究

植物名称普通小麦(Triticum aestivum L.)材料类别受精后二十天左右的胚乳。培养条件诱导愈伤组织采用 MS 培养基,附加2,4-D1.0ppm、NAA1.0ppm、6-BA0.2ppm、LH100ppm 和蔗糖5%。培养温度为26±1℃。分化芽培养基为 MS,附加6-BA2.0ppm、IAA0.5ppm、NAA1.0ppm、LH100ppm 和蔗糖5%。温度为26℃,光照400Lux、每日12小时照光。分化根培养基用 N_6 培养基     

唐菖蒲球茎芽的离体培养及快速繁殖

将带1-2个芽眼的唐菖蒲球茎切块接种到附加1.0mg/LBA的MS基本培养基上可诱导休眠芽萌动、无菌芽转移至附加3.0mg/LBA的培养基上可分化产生丛生芽。丛生芽的继代增殖宜采用附加1.5mg/LBA的培养基生根培养,以MS+NAA 0.1-0.5mg/L或MS+IBA 1.5mg/L效果最佳。试管苗移栽存活率可达50%左右。     

蛇床幼茎离体培养中体细胞胚胎形成的观察

蛇床幼茎外植体经诱导产生了愈伤组织。在ＭＳ＋２,４－Ｄ,０．２ｍｇ／Ｌ＋ＺＴ０．４ｍｇ／Ｌ培养基中,愈伤组织转变成胚性愈伤组织。转入ＭＳ＋ＮＡＡ０．２ｍｇ／Ｌ＋ＺＴ０．８ｍｇ／Ｌ培养基以后,胚性愈伤组织分化出体细胞胚胎。体细胞胚胎在ＭＳ＋ＮＡＡ０．５ｍｇ／Ｌ培养基中可直接发育成为完整植析。显微观察表明,体细胞胚胎产生于愈伤组织的表层细胞或内部细胞。在鱼雷胚期已有螺纹导管的分化。子叶期的维管组织从两     

In vitro organogenesis and plant regeneration from unpollinated ovary cultures of Azadirachta indica

A novel method of organogenesis in neem (Azadirachta indica A. Juss.) from unfertilized ovaries is described. The Murashige and Skoog’s (MS) medium with 9 % sucrose, 1 μM 2,4-dichlorophenoxyacetic acid (2,4-D) and 5 μM 6-benzylaminopurine (BAP) was the best for callus induction from unfertilized ovaries. However, further proliferation of callus occurred better on MS medium supplemented with 0.5 μM 2,4-D either alone or in combination with 4.5 μM kinetin. Maximum shoot regeneration (78 %) was observed when calli, induced from ovaries of 4 mm size flower buds and proliferating on MS + 0.5 μM 2,4-D, were subcultured to MS medium containing 5 μM BAP. Histological analysis revealed that 4 mm sized flower bud corresponds to a 2-nucleate stage of embryo sac. The shoots were then multiplied by forced axillary branching on MS medium supplemented with 1.0 μM BAP and 250 mg dm⁻³ casein hydrolysate. The shoots could be rooted on 1/4 strength MS medium supplemented with 0.5 μM indole-3-butyric acid (IBA) at a frequency of 79 %. Cytological analysis by root tip squash preparations revealed that all the plantlets were diploids. These plants were subsequently hardened and established in soil with transplantation rate of 81.8 %.     

In Vitro Induction of Haploid Plantlets from Unpollinated Young Ovaries of Lily and Its Embryo logical Observations

Unpollinated young ovaries of lily (Lilium davidii var. willmottiae (Wilson) Roffill) were inoculated on modified MS medium and N6 medium. Ovary cultures were incubated at 25–28℃, and illuminated with a fluorescent light of about 800–1200 Lux. Cultured ovaries gradually became thicker and longer after 10 days. The calli (about 6–12 mm in size) were produced after 40 days. The calli were then transferred to the differentiation medium. After 50 days, regeneration plantlets were formed. Embryoids were directly produced from some ovaries, which then developed into plantlets. Observation of chromosome number of regeneration plants shows: 65.71% regeneration plants are haploid plants, 34.29% are diploid. Embryological observation of ovary culture shows that haploid plants are from megaspore tetrad, while diploid plants are probably from nucellus cell.     

'早红'草莓高效遗传转化受体系统的建立

本文以草莓主栽品种'早红'组培苗离体叶片和叶柄为外植体,进行叶龄、暗培养、植物生长调节剂配比及抗生素敏感性研究,建立草莓高效遗传转化的受体系统.在含3.0 mg/L 6-BA与0.1 mg/L 2,4-D的MS培养基上,30 d叶龄的叶片再生频率高达98.31%,平均每叶片再生芽数5.09个,叶柄切段的再生频率为89.25%,平均每叶柄切段再生芽数4.92个,叶片的再生频率略高于叶柄;不定芽在含0.2 mg/L 6-BA与0.2 mg/L GA_3的MS继代培养基上培养成苗.将生长状态良好的不定芽转至含0.2 mg/L IBA的1/2 MS培养基上生根,生根率达100%,平均生根数量16.27条,平均根长1.85 cm.抗生素敏感性试验表明,草莓外植体适宜的卡那霉素选择压力为25 mg/L,头孢霉素的筛选浓度为300mg/L.本研究建立的再生体系可作为草莓遗传转化的受体系统.     

网纹瓜单细胞固-液双层培养及体细胞无性系建立(简报)

网纹瓜(Cucumis melo Var.reticulatus)是名贵的优质甜瓜,为葫芦科、甜瓜属植物。我国引种后生长良好,产量高,经济效益好,每年从日本购进大量杂交种子。但由于种子不纯,基因型差异较大,植株不整齐,产量不稳定,而且价格昂贵。因此,选育适合我国种植的     

Haploid induction via unfertilized ovary culture in watermelon

Unfertilized ovary culture constitutes an effective method for haploid breeding and can greatly shorten the breeding time. This method has been successfully used for breeding in many species, but reports of this method for breeding watermelon are scarce. Therefore, we performed an experiment to induce haploid plantlets. We evaluated the effects of several important factors on unfertilized ovary cultures of watermelon, including genotype, medium, the duration of induction and the development stage of the ovaries. The results revealed that the genotype of donor plants was a key factor for in vitro gynogenesis. The induction rate of eight watermelon cultivars varied from 0.00 to 15.14 ELSs per100 ovary slices. The most effective induction medium and maturation medium were MS medium supplemented with 3 mg L^??1 2,4-D, 2 mg L^??1 BAP, 0.5 mg L^?1 NAA and MS supplemented with 0.8 mg L^??1 BAP and 0.2 mg L^??1 NAA, respectively. The duration of induction significantly influenced ELS formation. The optimum duration was 13 days, and unfertilized ovaries collected at anthesis had the higher induction rate. We obtained more than 100 plantlets and used chromosome counting and flow cytometry to determine the ploidy levels of 50 of them, among which 48 were haploid and 2 were diploid. Our results demonstrated that in vitro gynogenesis can be induced in watermelon by unfertilized ovaries culture.     

发根农杆菌对骆驼刺的转化及转化组织的形态发生

将骆驼刺离体再生苗的茎切段经发根农杆菌A4菌株感染后,在含500mg/L头孢霉素的MS无激素培养基上培养,产生了转化的发根和愈伤组织.转化根在附加2mg/L2,4-D和0.5-1mg/L6BA的MS培养基上培养后,亦可诱导出愈伤组织.在含3mg/L6BA和0.5mg/LNAA的培养基上诱导出了苗的分化.冠瘿碱分析表明,在95%以上的发根和75%的转化愈伤组织及再生植株中都显示了T-DNA的整合和表达.染色体检查发现,约81%的发根细胞具有正常染色体数(2n=18),其余则存在染色体数目的变化,在继代培养一年之后,转化体仍维持旺盛的再生能力.