提高春小麦花粉植株诱导率的研究

本文研究了影响春小麦花粉植株诱导率的几种主要因素。供试材料为1990年温室种植的杂种F_1代,试验结果表明,诱导培养基中附加细胞分裂素BA或BA与KT相结合能显著提高愈伤组织分化率;0.17M的葡萄糖加0.17M的蔗糖比用0.26M的蔗糖愈伤组织诱导率高60％以上;愈伤组织在18～25℃比在23～25℃下培养绿苗率显著提高;接种前2～3℃预处理幼穗72小时对提高出愈率和绿苗分化率有明显效果。     

An improved method for dihaploid production in Nicotiana rustica through anther culture

Summary The efficiency of dihaploid production from anther culture in N. rustica has been improved by studying the effects of pretreatment temperature, pretreatment duration and initial anther stage on anther response, anther productivity and time to first plantlet production. Pretreatment was most effective on anthers at or around the stage of pollen mitosis. Pollen mitosis stage anthers pretreated at 9 °C for 15 days gave the best results. Both spontaneous and induced dihaploids were obtained. Small plantlets treated with 0.4% colchicine and 2% DMS solution for 5 h produced the maximum number of dihaploids (more than 50%). These considerable improvements in the efficiency of the techniques have made dihaploidy an attractive method for producing inbred lines in N. rustica. This will permit a large scale comparison of dihaploids with more conventional methods of inbreeding such as single seed descent and pedigree breeding.     

Expression of various gametic types in pollen plants regenerated from hybrids between Triticum-Agropyron and wheat

Summary Studies of the chromosomal composition of pollen plants regenerated from the F₁ of hybrids produced from Triticum-Agropyron intermediate type and common wheat demonstrated that various gametic types of the F₁ could be fully expressed at the whole plant level via anther culture. The observed frequency of each of the eight types of pollen plants (based on their chromosome numbers) was in good agreement with the theoretical probabilities as shown by X² analysis. Comparative studies of the chromosome composition of somatic cells and pollen mother cells (PMC's) of selected pollen plants permitted classification of the plants into four distinct classes. The majority of these regenerated pollen plants had identical chromosome numbers in both root tip cells and PMC's. An alien disomic addition line, which was cytologically stable for two generations, was obtained directly from anther culture. Moreover, the addition line exhibits resistance to stripe rust disease, a trait which is conferred by the Agropyron chromosome. We suggest that anther culture techniques provide a unique and expeditious route for the introduction of alien genes or chromosomes into wheat cultivars.     

甘蓝型油菜几个雄性不育系花药发育的细胞形态学研究

选用甘蓝型油菜6个细胞质雄性不育系和1个细胞核雄性不育系为材料,与可育系比较,确定花药发育受阻的时期和方式。根据研究结果,将其雄性不育系分为三类:1.湘矮A,Po-aA,陕2A和7s-3A花药发育受阻于孢原细胞分化期,没有分化形成花粉囊。2.萝AⅠ和萝AⅡ花药发育受阻于四分体至单核花粉期。败育方式为小孢子难以从四分体中释放出来,或释放出来后细胞质液泡化,核不能分裂,花粉壁发育不良。此外,还见到绒毡层径向肥大、延迟消失和维管束分化不良等异常现象。3.宜3A为核不育系,花药发育受阻于花粉母细胞期。败育方式为花粉母细胞死亡,减数分裂异常,或不能进行减数分裂。绒毡层和维管束一般都能正常发育。     

Somatic cell genetic studies inBrassica species

In vitro culture ofBrassica alba anthers on a growth medium containing inorganics of KB5 and organics, iron, sucrose and hormones of B5 resulted in a very high response of anthers (93.75%) towards callus induction. All the calli transferred to regeneration media responded favourably even after six months of callus induction. Numerous torpedo-shaped embryoids developed in clusters at many sites from each callus mass. Secondary embryogenesis and multiple shoot formation was also observed in many cases. The number of embryoids and plantlets produced by one embryogenic anther were as high as 169.8 and 17 respectively. 87% of the regenerated plants were haploids.     

Endothecial thickenings in the another wall ofPhthirusa adunca (Loranthaceae)

The thickenings in the anther wall ofPhthirusa adunca are confined to the endothecium. This observation resembles the previous report onP. pyrifolia.     

Absence of mitochondrial and chloroplast DNA recombinations in Brassica napus plants regenerated from protoplasts,protoplast fusions and anther culture

Summary Over 400 Brassica napus plants regenerated from individual protoplasts, from protoplast fusions and from anther culture were analysed for chloroplast and mitochondrial genome rearrangements by restriction fragment length polymorphisms. None were detected, attesting to the fidelity of the tissue culture procedures employed. In the majority of protoplast fusion products, the cytoplasmic organelles had completely sorted out at the callus stage but three regenerated plants possessed mixed parental populations of mitochondrial genomes and one regenerant contained mixed chloroplast genomes. In all four examples, the cytoplasmic genome sorted out in planta in favor of one parental type which was faithfully maternally transmitted to progeny.     

光对马来良姜花柱运动和花药开裂的影响

以马来良姜(Alpinia mutica)花柱为研究对象,研究光对花柱卷曲运动和花药开裂的影响.结果表明下垂型花柱的两次运动在光下和暗处都能进行,花药的开裂也不受光照影响.上举型花柱的第一次运动在暗处时向下进行,在光下时向上进行;暗处的花药不开裂,光下的花药开裂.第二次运动的方向和幅度取决于第一次运动期间的光照条件,第一次运动在暗处时,若第二次也在暗处,第二次运动不会发生且花药不开裂;若在光处,花柱向上运动.第一次运动在光下时,第二次运动无论光下或暗处,都向下运动.本研究表明,在不同光照条件下,两种表型的花柱与花药状态的组合使柱头接触不到同花的花粉,从而保证了雌雄异位与雌雄异熟.尽管两种表型的花柱运动和花药开裂行为相似,却受不同的机制调控.     

Microspore embryogenesis in barley: anther pre-treatment stimulates plant defence gene expression

Microspore embryogenesis (ME) is a process in which the gametophytic pollen programme of the microspore is reorientated towards a new embryo sporophytic programme. This process requires a stress treatment, usually performed in the anther or isolated microspores for several days. Despite the universal use of stress to induce ME, very few studies have addressed the physiological processes that occur in the anther during this step. To further understand the processes triggered by stress treatment, we followed the response of anthers by measuring the expression of stress-related genes in two barley (Hordeum vulgare L.) cultivars differing in their ME response. Genes encoding enzymes involved in oxidative stress (glutathione-S-transferase, GST; oxalate oxidase, OxO), in the synthesis of jasmonic acid (13-lipoxygenase, Lox; allene oxide cyclase, AOC; allene oxide synthase, AOS) and in the phenylpropanoid pathway (phenylalanine ammonia lyase, PAL), as well as those encoding PR proteins (Barwin, chitinase 2b, Chit 2b; glucanase, Gluc; basic pathogenesis-related protein 1, PR1; pathogenesis-related protein 10, PR10) were up-regulated in whole anthers upon stress treatment, indicating that anther perceives stress and reacts by triggering general plant defence mechanisms. In particular, both OxO and Chit 2b genes are good markers of anther reactivity owing to their high level of induction during the stress treatment. The effect of copper sulphate appeared to limit the expression of defence-related genes, which may be correlated with its positive effect on the yield of microspore embryos.     

Effect of growth regulators on microspore embryogenesis in coconut anthers

The effect of growth regulators on induction of androgenesis in coconut was investigated using seven different growth regulators at various concentrations and combinations. Three auxins (1-naphthalene acetic acid—NAA, indoleacetic acid—IAA, picloram) and three cytokinins (2-isopentyl adenine-2-iP, kinetin, zeatin) were tested either alone or in combination with 2,4-dichlorophenoxyacetic acid (2,4-D), using modified Eeuwens Y3 liquid medium as the basal medium. Among the tested auxins, 100 μM NAA in combination with 100 μM 2,4-D enhanced the production of calli/embryos (123) whereas IAA and picloram showed negative and detrimental effects, respectively, for androgenesis induction over 100 μM 2,4-D alone. Kinetin and 2-iP enhanced the production of calli/embryos when 100 μM 2,4-D was present in the culture medium. Both cytokinins at 10 μM yielded the highest frequencies of embryos (113 and 93, respectively) whereas zeatin (1 or 2.5 μM) had no impact on microspore embryogenesis. When calli/embryos (produced from different treatments in different experiments) were sub-cultured in somatic embryo induction medium (Y₃ medium containing 66 μM 2,4-D), followed by maturation medium (Y₃ medium without growth regulators) and germination medium (Y₃ medium containing 5 μM-6-benzyladenine—BA and 0.35 μM gibberellic acid—GA₃), plantlets were regenerated at low frequencies (in most treatments ranging from 0% to 7%).