High temperature enhances ethylene promotion of anther filament growth in Brussels sprouts (Brassica oleracea var. gemmifera)

A study was made of the effect of high temperature on the growth response of Brussels sprout filaments to ethylene. Filaments with or without the anthers attached were incubated continuously at 25 °C or 35 °C for 7 days or for 2 days at 35 °C followed by 5 days at 25 °C. Growth was reduced during both 35 °C treatments compared to that of filaments at continuous 25 °C. Ethylene had little effect on filament growth at continuous 25 °C, whereas with treatment for either 2 or 7 days at 35 °C ethylene promoted filament growth considerably. Thus ethylene effectively overcame the growth inhibition induced by the 35 °C treatment.High temperature treatments reduced ethylene production from filaments alone, and from filaments with anthers attached. The ethylene biosynthesis inhibitor aminoethoxyvinylglycine (AVG) and the ethylene action inhibitor AgNO₃ enhanced filament growth at 25 °C but had little or no effect at 35 °C. The relevance of temperature to ethylene sensitivity is discussed in relation to filament growth and to other plant processes in general.     

ABA promotion of ethylene production in anther culture of Brussels sprouts (Brassica oleracea var. gemmifera) and its relevance to embryogenesis

Abscisic acid (ABA) inhibited embryogenesis in anther culture of Brussels sprouts. This was accompanied by enhanced ethylene production during the first half of the anther culture period followed by a reduction in ethylene during the latter half, when compared to anthers not treated with ABA. The enhancement of ethylene production by ABA 6 h and 48 h after the start of the culture period was counteracted by the ethylene biosynthesis inhibitor aminoethoxyvinylglycine (AVG). Both AVG and the ethylene antagonist AgNO₃ removed much of the ABA inhibition of embryogenesis, suggesting that at least part of the ABA effect on embryo production is mediated through increased ethylene biosynthesis.
ABA promotion of ethylene production was reduced by high temperature: less ethylene evolved from ABA-treated anthers following a 24 h treatment at 35°C than from ABA-treated anthers incubated continuously at 25°C. A high temperature treatment such as this is invariably necessary for embryogenesis in Brussels sprouts anther culture.     

Effect of silver nitrate and 2,4-D on anther culture of Brussels sprouts (Brassica oleracea var. gemmifera)

The response to anther culture, of six genotypes of Brussels sprouts was tested on six media which included two levels of 2,4-D and the presence or absence of silver nitrate. The presence of silver was usually beneficial, and with some genotypes had a very large effect. Increasing 2,4-D could be beneficial in the absence of silver nitrate, but was sometimes detrimental in the presence of silver. Replacing agar with highly purified agarose was not particularly beneficial. Genotype, medium and genotype × medium interactions were all significant factors, with genotype being the most important.     

Anther culture in Brussels sprouts (Brassica oleracea var. gemmifera)

In Brussels sprouts, yields of up to 357 embryos per 100 anthers cultured were obtained using a thermal shock treatment of 16 h at 35°C at the start of the culture period. Treatments of 48 h at 35°C and 14 days at 30°C gave no embryos. The F₁ hybrid cv. Gower consistently gave higher embryo yields than the F₁ hybrid cv. Nym, the differences being 3 to 10-fold. Differences in embryo yield of 3-fold or less were usually not statistically significant because of great variation within a treatment. This variation was less with donor plants raised in a growth room than with those raised in a glasshouse, where temperature and light intensity could not be so accurately controlled. From 842 embryos cultured, 270 plants were regenerated, mostly via hypocotyl explants, which developed from the anther-derived embryos. Most of the regenerants were haploid or diploid, with a few of higher ploidy.     

Anther culture in Brussels sprouts (Brassica oleracea var. gemmifera).

Embryo yields from anther culture were determined for seven F₁ hybrid genotypes of Brussels sprouts, one of which was known to be highly responsive. At least 1400 anthers were cultured for each genotype and the genotypes were tested in two groups. Although the results were variable, the genotypes were provisionally grouped as follows: two were highly responsive (with up to 180 and 376 embryos per 100 anthers cultured), one was moderately responsive (with up to 53 embryos) and four were virtually non-responsive. The possible genetic basis for the difference in responsiveness is discussed, together with the implications of the results for the utilisation of anther culture in Brussels sprouts breeding.     

Ethylene production during anther culture of Brussels sprouts (Brassica oleracea var gemmifera) and its relationship with factors that affect embryo production

The ethylene inhibitor silver nitrate (AgNO₃) is known to overcome the poor response of the Brussels sprouts cultivar Hal to anther culture. Ethylene production by Hal anthers after 6 h of culture at 35°C was on average 10- and 20-fold greater than from anthers of the highly responsive cultivars Gower and GA1 x RDF2. The initial 24 h period at 35°C necessary for embryogenesis in anther culture of Brussels sprouts generally reduced ethylene production by the anthers after 6, 24, 48 and 72 h of culture, although the effect was not seen in 2 out of 3 Hal experiments until 24 h, and after 6 h was only found with 1 of 3 GA1 x RDF2 experiments. Embryo production was inhibited by the inclusion of the ethylene precursor, 1-aminocyclopropane-1-carboxylic acid (ACC) or the ethylene-releasing compound, ethephon in the media. Silver nitrate (AgNO₃) and the ethylene biosynthesis inhibitor aminoethoxyvinylglycine (AVG) promoted embryogenesis but did not substitute for the high temperature treatment. The relevance of ethylene production during anther culture to the effects of genotype and high temperature on anther culture embryogenesis is discussed.Abbreviations ACC 1-aminocyclopropane-1-carboxylic acid - AVG aminoethoxyvinylglycine     

Genetic and non-genetic factors affecting anther culture of Brussels sprouts (Brassica oleracea var. gemmifera)

Summary Eight inbred lines of Brussels sprouts and ten F₁ hybrids derived from them were tested for their response to anther culture. From 5–19 plants per genotype were tested, and each plant was tested on 3–6 separate occasions. Results from the inbred lines were broadly similar to those from the F₁ hybrids, despite the inbreds producing fewer buds and having a higher frequency of anther deformities. The maximum embryo yield from an inbred line was 215 embryos per 100 anthers, and from a hybrid was 275. From estimation of the variance components it was calculated that, for both inbreds and hybrids, about half the total variation was genetic whereas variation due to plants within genotypes and to occasions within plants were each about 13% of the total. The narrow sense heritability of responsiveness to anther culture (estimated by the proportion of variation between inbred lines which was genetic) was 0.48, and there was partial dominance for this character. In three cases the hybrid outyielded the better inbred, and this heterosis may well be due to dispersed dominant genes.     

The feasibility of producing inbred rather than F1 hybrid cultivars in Brussels sprouts (Brassica oleracea var. gemmifera): an assessment of recombinant inbred lines

Results are presented for the performance of improved inbred lines of Brussels sprouts grown in replicated and fully guarded plots. Some lines were identified which out-performed the reference F₁ hybrid, Gower, for the yield of marketable sprouts and for sprout quality. No lines were found which were superior for both of these traits. These results support earlier contentions that inbred line performance in Brussels sprouts could be improved to levels comparable with those of commercial F₁ hybrids. The genetic gains required to achieve commercial parity with hybrids for all agronomically important traits continue to be large. Therefore, the use of inbred lines as commercial cultivars can only be viewed as a long term objective. Previous studies have identified additive x additive epistasis and the segregation of many loci as important factors limiting the genetic gains to be expected from a single cycle of crossing and inbreeding. In addition to these factors the current study identifies areas of difficulty encountered when attempting to screen and select large numbers of inbred lines, produced either by single seed descent or by anther culture, in a single season. Evidence is presented which suggests that imperfect visual selection and/or genotype × seasonal interactions may substantially reduce the efficiency of selections based upon a single trial of very many unreplicated lines.     

Root growth dynamics of Brussels sprouts (Brassica olearacea var.gemmifera) and leeks (Allium porrum L.) as reflected by root length,root colour and UV fluorescence

Minirhizotron observations of roots of leeks and Brussels sprouts grown in the Wageningen Rhizolab were used to study the dynamics of root length. Day of appearance and the time of decay were assessed for individual root segments visible on the minirhizotron surface.A Brussels sprouts crop produced much more root length than leeks, but the average longevity of these roots was about half that of leek roots.To investigate whether root colour or UV fluorescence could be used as a quantitative index of root functionality or root age, changes in root colour (on a scale of greys) over time were measured with interactive image analysis. In both crops a gradual change towards black was found with ageing. Measurements of the intensity of the UV fluorescence showed that leek roots fluoresced more than Brussels sprouts roots. Over time, UV fluorescence decreased in Brussels sprouts roots but increased in leek roots. It is concluded that UV fluorescence cannot be used as a universal indicator of root age or root functionality, but in some plant species it may be used to separate (transparent) roots from the background with image analysis techniques.     

Molecular cloning, characterization and analysis of the intracellular localization of a water-soluble Chl-binding protein from Brussels sprouts (Brassica oleracea var. gemmifera)

A water-soluble Chl-binding protein from Brussels sprouts (Brassica oleracea var. gemmifera), hereafter termed BoWSCP, is categorized into the Class II WSCPs (non-photoconvertible WSCPs). Previous studies on BoWSCP have focused mainly on its biochemical characterization. In this study, we cloned the cDNA encoding BoWSCP. Sequence analysis revealed that the BoWSCP gene was composed of a single exon corresponding to 654 bp of an open reading frame encoding 218 amino acid residues, including 19 residues of a deduced signal peptide targeted to the endoplasmic reticulum (ER). Matrix-assisted laser desorption ionization time-of-flight mass spectrometry analysis of native BoWSCP revealed that the molecular mass of the subunit was 19,008.523 Da, corresponding to a mature protein of 178 amino acids, indicating the removal of 21 residues in the C-terminal region. Functional BoWSCP was expressed in Escherichia coli as a hexa-histidine fusion protein (BoWSCP-His). When BoWSCP-His was mixed with thylakoid membranes in aqueous solution, BoWSCP-His was able to remove Chls from the thylakoid membranes. The absorption spectrum of the reconstituted BoWSCP-His was identical to that of the native BoWSCP. Chl binding analyses of BoWSCP-His revealed that the BoWSCP-His bound both Chl a and Chl b with almost the same affinity in 40% methanol solution, although the native BoWSCP had a higher content of Chl a. To reveal the intracellular localization of BoWSCP, we constructed a transgenic plant expressing the fluorescent protein fused with the N-terminal deduced signal peptide of BoWSCP. The fluorescence emitted from the chimeric protein was detected in the ER body, an ER-derived compartment observed only in Brassicaceae plants.     

The Effect of Rooting Space on Whole Plant and Leaf Growth in Brussels Sprouts (Brassica oleracea var. gemmifera)

Seedlings of Brassica oleracea var. gemmifera DC. (Brusselssprouts) were grown in four pot sizes over a 4-week period.Whole plant, stem, root and foliage d. wts and foliage area,together with specific leaf area, leaf area ratio and numberof leaves initiated were reduced by restricting rooting space.Individual leaves showed similar reductions in d. wt and area,with the effect being more pronounced in later-formed leaves.Cell counts and measurements on the epidermis and palisade mesophylllayers of the first four leaves showed that the reduction ingrowth was due to reduced cell division. Cell numbers in thefirst-formed leaf were halved over the range of pot sizes used,and there was a progressively greater reduction in cell numbersin later-formed leaves. There was some tendency for cell sizeto decrease with decreasing rooting space, but this was notgeneral and was most marked between plants grown in the twosmallest pot sizes. Brassica oleracea var. gemmifera, Brussels sprouts, rooting space, growth analysis, leaf growth, cell numbers, cell sizes     

The Distribution of Hormones in Relation to Apical Dominance in Brussels Sprouts (Brassica oleracea var. gemmifera L.) Plants

The lateral buds of intact Brussels sprout plants containedless auxin and gibberellin than the main apex. When the apexwas removed the auxin content of the top lateral buds increasedwithin 2 days, but gibberellin activity did not increaseuntilshoot extension was apparent. Auxin application to the cut surfaceof decapitated plants caused lateral bud inhibition, but didnot completely prevent bud growth. Both auxin and gibberellinactivity in the plant apex decreased with increasing age, butonly gibberellin activity decreased in the lateral buds. Theauxin content of the lateral buds on intact plants increasedwith time. It is suggested that in Brussels sprouts, lateral bud inhibitionis due to sub-optimal auxin activity, and that decapitationinduces an auxin increase in these buds which then grow out.Lateral shoots are produced following decapitation of youngplants because the gibberellin content of the lateral buds isrelatively high. Only bud swelling occurs in decapitated olderplants because the gibberellin content of the buds is too lowto stimulate shoot extension. It is concluded that these results support the theory that hormone-inducednutrient diversion may control lateral bud development.     

The Production of Plantlets from Tissue Cultures of Brussels Sprout (Brassica oleracea L. var gemmifera D.C.)

Shoots were induced on callus derived from sprout sections andpetiole slices of an inbred parent line of Brussels sprout (Brassicaoleracea L. var gemmifera D.C.). The shoots, when excised andtransferred to fresh medium, enlarged and formed roots. Theseplantlets could be transferred to soil or their number increasedby a multiplication process involving the production of newshoots from the dormant lateral buds. Some of the plantletsderived from sprout callus were grown to maturity in the fieldand their morphology and chromosome number compared to seedgrown plants. There were no significant differences in sproutsize and stem diameter but there were significant differencesin plant shape. None of the plants in the field experiment showedpolyploidy. Plants derived from callus possessed an enhanced ability toform callus and redifferentiate when sections from these plantswere placed back on to nutrient medium.     

组织培养法快速繁殖抱子甘蓝F1植株

1　植物名称　抱子甘蓝 (Ｂｒａｓｓｉｃａｏｌｅｒａｃｅａｖａｒ Ｚｅｎｋ ｇｅｍｍｉｆｅｒａ)。2　材料类别　荷兰Ｎｏｖａｒｌｉｓ公司培育的“绿橄榄”Ｆ1 代种子萌发后幼苗的下胚轴。3　培养条件　 (1 )播种培养基 :1 /2ＭＳ 0 6 5 %琼脂 3 %蔗糖。 (2 )诱导培养基 :ＭＳ 6 ＢＡ 2ｍｇ·Ｌ- 1 (单位下同 ) 0 8%琼脂 3 %蔗糖 ;扩增培养基 :ＭＳ 6 ＢＡ 4 0 8%琼脂 3 %蔗糖。 (3 )生根培养基 :不含激素的ＭＳ培养基。ｐＨ 5 8,温度为 2 5℃ ,光照度 1 5 0 0ｌｘ,光照时间 1 4ｈ·ｄ- 1 。4　生长与分化情况4.1　种子无菌…     

Variations in response to high temperature treatments in anther culture of Brussels sprouts

The level, time of application and duration of the high temperature treatment necessary for embryo production from Brussels sprouts anther culture were examined. The effects of 29, 32, 35, and 38°C given for 24 h immediately following removal of the anthers from the bud, were tested on different cultivars, on different plants within the cultivars and on different occasions for each plant. Most embryos were produced following 32 and 35°C, very few following 30°C and none following 38°C. Although there was a tendency for some cultivars to respond better to one or other of the two more favourable temperatures, this varied considerably between individual plants. Plant to plant variation was also seen in the overall level of the response, although responsiveness tended to decline with successive samplings of the same plant. Experiments with cultivars Hal and Gower suggested that high temperature was required for at least 12 h after anther removal, but beyond that time the optimum period varied from plant to plant. If the excised anthers were held at 25°C for 16 h or more with Hal or 24 h or more with Gower before being exposed to the high temperature treatment, embrogenesis tended to be reduced. It is suggested that apparent non-responsiveness in anther culture may result to a large extent from the specific conditions that are used during the anther culture process.     

Differences in red cell shape of two inbred chicken lines

Summary Comparison of two inbred chicken lines (F_x > 99.9%) revealed significant differences in shape of the red blood cells (RBC). The length-width index was lower for both sexes in IC-line (1.46) when compared to CB-line chickens (1.88). Phenotypic expression of this character in F₁ hybrids and both backcross groups corresponded to the common manifestations of the metric parameters. The index in F₁ hybrid chickens deviated from intermediate values with the dominant tendency to oval RBC. An analysis of the segregating first backcross generation chickens did not show any association between RBC shape and the genotype in the blood group systems B, C, I, and D and the IgG allotypes. The differences in RBC shape were probably not associated with the survival of RBC in the blood circulation.     

Distribution of elemental interactions in Brussels sprouts plants,under the Treated Municipal Wastewater

Abstract

The distribution of the macro, micronutrients and heavy metal interactions in the various plant parts (roots, leaf, and sprout) of Brassica oleracea var. gemmifera (Brussels sprouts), was investigated in a greenhouse experiment of randomized block design, in Agrinion, Greece. The statistical design included two variables: (i) Treated Municipal Wastewater (TMWW), and (ii) fresh irrigation well water (control). The analytical data of plant and soil samples collected were processed statistically by means of regression analysis, ANOVA and t-test, using an SPSS package. The ultimate goal of the experiment was to establish a scientific basis for the safe re-use of TMWW in the irrigation of Brussels sprouts, and possibly of all vegetables, with least accumulation of heavy metals in the sprouts.     

结球甘蓝和青花菜小孢子胚植株再生

结球甘蓝(Brassica oleracea var. capitata)和青花菜(Brassica oleracea var. italica)小孢子胚再生植株频率低是目前影响游离小孢子培养技术有效应用的关键问题之一, 研究其小孢子胚植株再生频率的影响因素, 提高胚再生植株频率, 对促进游离小孢子培养技术在甘蓝类蔬菜育种中更好地应用具有重要意义。该文以结球甘蓝中甘11和青花菜TI-111等基因型为试材, 对影响游离小孢子胚再生成植株的固体培养基类型、琼脂浓度、胚的类型及胚在液体培养基中的滞留时间等因素进行了研究。结果表明: 游离小孢子培养25天的子叶胚在琼脂浓度为1%–1.25%的B5培养基上植株再生频率最高。进一步通过8个不同基因型对上述实验结果进行了验证, 结果显示, 游离小孢子培养25天的子叶胚在1%琼脂浓度的B5培养基上植株再生频率达77.8%–97.2%。     

结球甘蓝和青花菜小孢子胚植株再生

结球甘蓝（Brassica oleracea var.capitata）和青花菜（Brassica oleracea var.italica）小孢子胚再生植株频率低是目前影响游离小孢子培养技术有效应用的关键问题之一,研究其小孢子胚植株再生频率的影响因素,提高胚再生植株频率,对促进游离小孢子培养技术在甘蓝类蔬菜育种中更好地应用具有重要意义。该文以结球甘蓝中甘11和青花菜TI-111等基因型为试材,对影响游离小孢子胚再生成植株的固体培养基类型、琼脂浓度、胚的类型及胚在液体培养基中的滞留时间等因素进行了研究。结果表明：游离小孢子培养25天的子叶胚在琼脂浓度为1%–1.25%的B5培养基上植株再生频率最高。进一步通过8个不同基因型对上述实验结果进行了验证,结果显示,游离小孢子培养25天的子叶胚在1%琼脂浓度的B5培养基上植株再生频率达77.8%–97.2%。     

Effect of silver nitrate on long-term culture and regeneration of callus from Brassica oleracea var. gemmifera

Incorporation of AgNO₃ (1–10 mg1^-1) into the culture medium of Brassica oleracea var. gemmifera callus significantly improved growth and allowed long-term callus culture. In the absence of AgNO₃, callus died shortly after removal from the hypocotyl explants. Regeneration of shoots from callus on low-hormone medium was also enhanced by AgNO₃. Significant differences in shoot production were found between the three genotypes examined. Cv. Aries produced large numbers of shoots even in the absence of AgNO₃. Investigation of callus production from the inbred parent lines of cv. Aries indicated that tissue culturability may be determined genetically.Abbreviations 2,4-D 2,4-dichlorophenoxyacetic acid - NAA naphthaleneacetic acid