Differentiation of Non-articulated Laticifers in Poinsettia (Euphorbia pulcherrima Willd.)

Differentiation of non-articulated laticifers in poinsettia(Euphorbia pulcherrima Willd.) was studied ultra-structurally.Growing laticifers show: (1) a multinucleate apical region containingabundant ribosomes but few other differentiated organelles and(2) a sub-apical zone where the cytoplasm is dominated by vacuolesof diverse morphology with latex particles. These particlesappear first within narrow tubular vacuoles developed especiallyin the peripheral cytoplasm. During vacuolation of the laticifer,portions of cytoplasm, including some of the nuclei, becomeisolated by the enlarging and fusing vacuoles; eventually thesebecome lysed, except the latex particles which remain in thecentral vacuole. During differentiation of a laticifer branch,the cytoplasm contains the usual organelles, including a fewmicrobodies and coated vesicles. The plastids that lie withinthe peripheral cytoplasm differentiate into amyloplasts witha single elongated starch grain. Towards the end of differentiationthe cytoplasm becomes restricted to a thin parietal layer, withthe remaining organelles reduced or degenerate, surroundinga central vacuole filled with latex particles. Euphorbia pulcherrima Willd, poinsettia, ultrastructure, differentiation, laticifers     

Ethylene Evolution from Bracts and Leaves of Poinsettia, Euphorbia pulcherrima Willd

Woodrow, L. and Grodzinski, B. 1987. Ethylene evolution trombracts and leaves ol Poinsettia, Euphorbia pulcherrima Willd.—J.exp. Bot. 38: 2024–2032. Ethylene release from fully expanded, red and white bracts andleaves of poinsettia, Euphorbia pulcherrima Willd., was compared.On a laminar (area) basis leaves contained about 50 times morechlorophyll and demonstrated 10 times the photosynthetic rateof the bracts. Both tissues contained starch, however, solublecarbohydrate in the bracts consisted primarily of reducing hexoseswhile the leaves contained mainly sucrose for translocation.The total free alpha-amino nitrogen content of the bract tissuewas twice that of the leaf tissue. The leaves contained moreACC (1-aminocyclopropane-1-carboxylic acid) and produced proportionallymore endogenous C²H⁴ than either the red or white bracts. ACC-stimulated₂H₄ release was also greatest from the green tissue indicatingthat the EFE (ethylene forming enzyme) was most active in theleaves. The specific activity of the ¹⁴C₂H₄/¹²C₂H₄ releasedfrom [2,3-¹⁴C]ACC confirmed ACC as the primary precursor ofC₂H₄ in this tissue. Ethylene release from the non-photosynthetic,bract tissue was not markedly affected by alterations in CO₂or light conditions. In green leaf tissue endogeneous ethylenerelease increased from 1·5 to 6·0 pmol C₂H₄ cm^–2h^–1 while ACC-stimulated ethylene release increased from10 to 35 pmol C₂H₄ cm^2– h^1– as the CO₂ partial pressureincreased from 100 to 1 200 µbar. Key words: Poinsettia, ethylene, bracts     

Distribution and Organization of Non-articulated Laticifers in Mature Tissues of Poinsettia (Euphorbia pulcherrima Willd.)

The distribution and cytological organization of non-articulatedbranched laticifers in the mature root, stem, and leaf tissuesof poinsettia. Euphorbia pulcherrima Willd., were studied bythe use of optical and electron microscopy. The laticifers occurin all parts of the plant body, being well represented in certainparenchymatous tissues and the phloem. The mature region ofthe laticifer has a living protoplast showing a thin parietalcytoplasm, bounded by plasmalemma and a tonoplast, which enclosesa large continuous central vacuole containing the milky latexfluid. The protoplast is multinucleate and possesses large amyloplasts,each enclosing a single elongated starch grain. Sparseness andpoor differentiation of the other components of the protoplast,mostly mitochondria, ribosomes and endoplasmic reticulum, suggestlow metabolism in the mature region of the laticifer. The latexof the central vacuole is dominated by spherical particles,0.3–1 µm in diameter, each with a dense matrix andan eccentric core of lighter staining material. In some laticifersthe latex particles fuse into coagulated masses. Euphorbia pulcherrima Willd, poinsettia, laticifers, ultrastructure, cytology     

一品红花色素抗氧化性能的研究

从一品红红色苞片中提取花色素,并用自由基测定试剂盒测试了一品红花色素的体外抗氧化性能,并用碘量法测定了其抑制猪油氧化的效果,用TBARS法测定其对血浆脂蛋白氧化的抑制能力。结果表明:一品红花色素具有较强的清除超氧阴离子(O2.-)和羟自由基(.OH)的能力,清除效果优于同浓度的VC;其对猪油氧化的抑制效果和同浓度的VC相近,而对人血浆脂质过氧化的抑制效果显著高于VC。     

一品红体细胞胚胎发生与植株再生

一品红不同部位愈伤组织诱导能力存在差异,嫩茎>幼花序>嫩叶。愈伤组织的长势主要受生长素的影响,细胞分裂素对愈伤组织生长有促进作用;但在含6-BA和NAA的培养基中诱导出的愈伤组织,其胚性明显强于单独用NAA诱导出的愈伤组织。液体悬浮培养是一品红体细胞胚胎高频发生的中间步骤。不同浓度BA对一品红体细胞胚的萌发率影响不大,萌发培养基中KNO₃含量加倍可提高萌发率。     

一品红苞片花色素的分离及初步鉴定

用紫外-可见光分光光度计、高效液相色谱(HPLC)和质谱(MS)技术对一品红(Euphorbia pulcherrima)红色苞片中的花色素提取液进行了初步鉴定。一品红花色素的甲醇溶液分别在270、340 和520 nm 处有 3 个吸收峰; 在 440 nm 吸光度与可见光最大吸收波长 520 nm 吸光度的比值 为0.29; 花色素的甲醇溶液中加入AlCl3后发生红移, 再加入HCl后发生蓝移; 色素溶液在紫外光下无荧光; 色素样品经液相色谱分离后在 270 nm检测有 5 个比较明显的吸收峰; 质谱中得到 595、611、381、571 和 589 等对应的分子离子峰; 花色素酸解液高效液相色谱图谱和鼠李糖、葡萄糖的出峰时间一致。由这些结果可推断一品红花色素样品中主要含有 5 种组分: 矢车菊花色素芸香苷、飞燕草花色素芸香苷、飞燕草花色素苯甲酰基葡糖苷、矢车菊花色素苯甲酰基葡糖苷和一种未知成分。     

一品红苞片花色素的分离及初步鉴定

用紫外-可见光分光光度计、高效液相色谱（HPLC）和质谱（MS）技术对一品红（Euphorbia pulcherrima）红色苞片中的花色素提取液进行了初步鉴定.一品红花色素的甲醇溶液分别在270、340和520 nm处有3个吸收峰;在440 nm吸光度与可见光最大吸收波长520 nm吸光度的比值为0.29;花色素的甲醇溶液中加入AlCl3后发生红移,再加入HCl后发生蓝移;色素溶液在紫外光下无荧光;色素样品经液相色谱分离后在270 nm检测有5个比较明显的吸收峰;质谱中得到595、611、381、571和589等对应的分子离子峰;花色素酸解液高效液相色谱图谱和鼠李糖、葡萄糖的出峰时间一致.由这些结果可推断一品红花色素样品中主要含有5种组分：矢车菊花色素芸香苷、飞燕草花色素芸香苷、飞燕草花色素苯甲酰基葡糖苷、矢车菊花色素苯甲酰基葡糖苷和一种未知成分.     

外源表达的人copine V诱导细胞死亡的研究

目的：copines蛋白家族是新近发现的一类分布广泛、进化保守的Ca2＋依赖性磷脂结合蛋白,copineV是其成员之一.为研究copineV基因的功能,构建了人copineV基因的真核表达质粒并转染HEK293细胞,以进一步研究其功能.方法：构建人copineV编码区序列的真核表达质粒pCDNA4/copineV,脂质体法转染HEK293细胞.通过RT-PCR、克隆形成实验和Hochesst33342染色等方法观察copineV基因对HEK293细胞生长的影响.结果：外源表达的人copine V可以诱导HEK293细胞死亡,无法筛选到稳定克隆.结论：人copineV可以诱导HEK293细胞死亡,为进一步研究copineV基因的生物功能提供了线索.     

Parallelism in hill activity and anthocyanidin content in Euphorbia pulcherrima

Pigment compositions and Hill activities of red-leafy bracts, red-green leaves and green leaves of E. pulcherrima were studied. Interestingly enough, the chloroplasts from anthocyanidin-containing leaves are intrinsically more active than those from green leaves.     

Sterols and triterpenols in latex and cultured tissues of Euphorbia pulcherrima

The sterol and triterpenol constituents of Euphorbia pulcherrima latex and cultured callus tissues were examined by GLC and mass spectrometry. Latex extracts from different varieties contained sitosterol, β-amyrin, germanicol, cycloartenol, β-amyrin acetate, and germanicol acetate. Capillary GC profiles of these varieties indicated that the triterpene content was essentially identical for examined latices. Cultured tissues derived from petioles and stem internodes synthesized only sitosterol in significant quantities, although trace amounts of several sterols that occur in latex were also detected in cultured tissues. This study supports the interpretation that the pattern of triterpene synthesis in the laticifer of the normal plant is a highly controlled and stable phenomenon among varieties of this species.     

Molecular Characterization of a Distinct Begomovirus Infecting Euphorbia pulcherrima in China

Virus isolate G35 was obtained from Euphorbia pulcherrima showing leaf curl and vein thickening symptoms in Tianyang, Guangxi Province, China. The virus was transmitted by whiteflies to Nicotiana tabacum, Lycopersicon esculentum, Datura stramonium and E. pulcherrima. DNA‐A contains 2746 nucleotides, with two open reading frames (ORFs) in the virion‐sense DNA and four ORFs in the complementary‐sense DNA. When compared with the DNA‐A sequence of other begomoviruses, the total DNA‐A of isolate G35 was most closely related to that of Ageratum enation virus (79.9% sequence identity). However, the deduced coat protein of G35 is most like that of Pepper leaf curl virus from Bangladesh (94.9% amino acid sequence identity), and the AC1 of G35 is most like that of Cotton leaf curl Multan virus‐Okra (87.2% amino acid sequence identity). The molecular data showed that G35 is a distinct Begomovirus species, for which the name Euphorbia leaf curl virus (ELCV) is proposed.     

Arabinogalactan proteins in embryogenic and non-embryogenic callus cultures of Euphorbia pulcherrima

The arabinogalactan protein (AGP) fractions of embryogenic and non-embryogenic callus lines of Euphorbia pulcherrima Willd. ex. Klotzsch were analysed over a cultivation period of 9 weeks using the β -glucosyl Yariv reagent and an anti-AGP antibody (LM2). The amount of AGPs detected with the Yariv reagent increased in embryogenic cultures during the development of somatic embryos. The embryogenic and non-embryogenic callus contained different sets of AGPs characterized with the Yariv reagent and the LM2 monoclonal antibody. AGPs recognized by LM2 are localized primarily in the protodermal cells of globular somatic embryos. The development of somatic embryos of E. pulcherrima appears to be associated with the presence of particular AGPs.     

一品红叶片的组织培养及其植株再生(简报)

一品红叶片外植体在MS IAA0．4mg／L 6-BA4．0mg／L的培养基上培养15d后产生疏松的浅绿色愈伤组织,30d后开始从愈伤组织表面分化产生幼芽,45d后平均每块愈伤组织产生15株幼芽。将幼芽转至含0．5mg／LIBA的MS培养基上形成根,再形成完整植株。     

矮生一品红试管快速繁殖技术研究

矮委一品红试管苗增殖的最佳培养基为MS 6-BA0.2mg/L NAA0.05mg/L 0.36%琼脂,每月增殖倍数7.6,最佳生根培养基为1/4MS IBA1.0mg/L 琼脂0.36g/L,每株生根2～3条,试管苗移栽成活率86.5%。     

Polyphenoloxidase-activity and -activation in embryogenic and non-embryogenic suspension cultures of Euphorbia pulcherrima

The activity and activation potential of polyphenoloxidase (PPO, E.C. 1.10.3.1.) of tissue from shoot tips, adult leaves and embryogenic and non-embryogenic cell suspension cultures of Euphorbia pulcherrima was investigated using an oxygen probe technique. PPO derived from differentiated in vivo plant tissue (shoot tips, leaves) cannot be activated either by storage at 0–4°, freezing and thawing, incubation with CaCl₂, sodium dodecyl sulfate or by incubation with trypsin. Embryogenic cells are characterized by high initial PPO activity and strong activation potential of membrane bound enzyme. Non-embryogenic material reveals low phenolase activity and low activation potential. An activation quotient (based on the ratio between PPO-activity determined after sodium dodecyl sulfate incubation to PPO-activity determined after CaCl₂-incubation) was calculated. This is independent of absolute enzyme activity and can be used for characterization of the embryogenic status of cells.Abbreviations fw fresh weight - MS Murashige and Skoog - PPO polyphenoloxidase - SDS sodium dodecyl sulfate     

Differences in compounds released by embryogenic and non-embryogenic suspension cultures of Euphorbia pulcherrima

Media from embryogenic and non-embryogenic cell suspension cultures were analysed for protein content, electrophoretic protein patterns, glycoproteins and activity of peroxidases and β-glucosidases in order to characterize the physiological status of the cultures. On a dry mass basis the amount of extracellular proteins per cell was greater in embryogenic suspensions than in non-embryogenic suspensions. Non-embryogenic suspensions contained unidentified slimy compounds which were not present inembryogenic cultures. The extracellular Concanavalin A-specific glycoproteins gave different isoelectric focussing patterns and thus enabled embryogenic and non-embryogenic cultures to be differentiated. The extracellular peroxidase activity per cell dry mass was far greater in embryogenic than in non-embryogenic cultures. The isoenzymes differed in number and composition of the anionic bands. β-glucosidases were found in the same range of activity in both culture types, but the time course of enzyme activity during cultivation was significantly different. In the embryogenic culture the activity was correlated with dry mass increase, whereas in the non-embryogenic suspension the activity reached maximum during the linear growth phase. Polyphenoloxidase which was recently recognized as an intracellular marker for embryogenic stages was not released into culture media. This revised version was published online in July 2006 with corrections to the Cover Date.     

一品红试管苗移栽驯化期叶片的解剖结构变化

对一品红试管苗移栽驯化,同时研究了驯化过程中叶片结构的变化,结果表明,一品红在珍珠岩基质中成活率达98%,随着移栽时间的延长,表皮细胞增大,排列紧密;叶肉细胞间隙减小,栅栏组织细胞长度增加,主脉增厚,导管数目增加,保水,输水和抗逆能力增强。     

钙肥对B型烟粉虱发育、存活及取食为害的影响

以清水为对照,研究了施用钙肥后一品红植株对B型烟粉虱发育、存活和取食为害的影响.结果表明:在温度(26±1)℃、相对湿度60％～80％条件下,钙肥处理的一品红植株上的B型烟粉虱在发育历期上与对照存在显著差异,卵期明显缩短,各龄若虫期延长,从卵到成虫的发育时间为20.18 d,而对照为18.72 d;但钙肥处理对B型烟粉虱各虫态的存活率无显著影响.B型烟粉虱的取食为害诱导了一品红叶片叶绿素荧光参数的变化,显著降低了叶片的光合作用能力,其中光化学效率(Fv/Fm)、光化学淬灭系数(qp)、光能利用效率(α)、最大光合速率(rETRmax)以及对光的耐受能力(Ik)显著降低,而非光化学淬灭系数(NPQ)显著增加.钙肥处理一品红受害叶片的光抑制参数(β)、rETRmax和Ik水平与对照相当.通过指甲油印迹法观察叶片下表皮细胞的形态结构发现,钙肥能有效增强叶片对B型烟粉虱为害损失的补偿.     

Axillary Bud Inhibition Induced by Young Leaves or Bract in Euphorbia pulcherrima Willd

In plants held under long days in the vegetative stage, youngexpanding leaves of poinsettia (Euphorbia pulcherrima Willd.‘Brilliant Diamond’) are the main source of axillarybud inhibition, while the apical bud, which includes the meristem,primordial leaves and small unfolded leaves, is a secondaryinhibition source. Removal of these expanding leaves resultedin rapid release and growth of axillary buds. Decapitation ofthe apical bud resulted in delayed axillary bud release. Inreproductive plants kept in short days, the pigmented bractsare the primary source of axillary bud inhibition and the cyathiaare the secondary source. Applications of NAA —substitutedfor both young leaves and bract inhibition — maintainedapical dominance. The concentration of endogenous auxin washighest in the apical bud. However, when calculated on wholeorgan basis the auxin level was greater in young developingvegetative leaves and in reproductive bracts than in the apicalbud. Euphorbia pulcherrima Willd, apical bud, apical dominance, auxin, correlative inhibition, cyathia, poinsettia, IAA, NAA