植物生长延缓剂的生化效应

植物生长延缓剂的生化功能主要是抑制GA的生物合成。根据抑制的位置,分成类化合物（抑制GGPP转变为内根-贝壳杉烯的过程）、含氮杂环化合物（抑制内根-贝壳杉烯转变为内根-贝壳杉烯酸的过程）和酰基环己烷二酮（抑制GA12醛转变为GA8的过程）等三类。某些植物生长延缓剂还有抑制甾醇生物合成,影响ABA、乙烯、多胺及细胞分裂素代谢等副作用。     

高等植物赤霉素2-氧化酶基因的克隆、表达及其调控

赤霉素(GA)是一类重要的植物激素,对高等植物整个生命周期的生长发育起关键作用。调控赤霉素生物合成和代谢途径中的关键酶基因的表达可以控制植物体内赤霉素的含量。GA2-氧化酶是调节赤霉素合成和代谢的关键酶之一,使活性GA失活。本文主要对GA2-氧化酶基因的克隆、表达调控及其在植物基因工程中的应用等方面进行综述,为通过基因工程技术调控植物体内活性赤霉素的含量从而得到改良品种提供思路。     

赤霉素调节植物对非生物逆境的耐性

赤霉素（GAs）是一类重要的植物激素,调控植物生长发育的诸多方面．最近的研究表明,GA也参与对生物与非生物胁迫的响应,然而GA参与非生物胁迫响应的遗传学证据及其机制有待于进一步研究．本实验室前期研究证明,水稻EullfELONGATEDUPPERMOSTINTERNODE）通过一个新的生化途径降解体内的活性赤霉素分子,并参与调控水稻对病原菌的基础抗病性．本研究发现,euil突变体对盐胁迫能力降低,而超表达EUll基因的水稻和拟南芥耐盐性显著提高．进一步研究发现,积累高含量赤霉素的水稻euil突变体对脱落酸（ABA）的敏感性下降,而赤霉素缺失的EUll超表达转基因水稻和拟南芥均改变了对于ABA的敏感性．EUll基因的转录受逆境诱导,其功能缺失与超表达调控了逆境标志基因的表达．综上推测,GA可能是通过影响ABA的信号途径从而改变了植物对非生物胁迫的响应．     

甜菊醇糖苷生物合成及关键酶研究进展

甜菊醇糖苷(steviol glycosides,SGs)是甜叶(Stevia rebaudian)叶片中一类天然甜味剂,具有高甜度、低热量、无毒副作用等特点,同时还具有一定的药理作用.植物体内主要是通过甲基赤藓糖醇(MEP)途径形成祝(牛)儿(牦)牛儿焦磷酸(GGPP),之后该物质在古巴焦磷酸合酶(CPPS)、贝壳杉烯合酶(KS)、贝壳杉烯氧化酶(KO)、糖菊苷转移酶(UGTs)等一系列结构功能各异的酶的作用下最终生成甜菊醇糖苷.SGs生物合成途径的调控及该途径中关键酶的研究已成为目前国内外生物学领域的一大热点.综述了甜叶菊SGs生物合成途径和参与该途径中的关键酶及其基因的研究进展,并展望了其应用前景.     

高等植物赤霉素生物合成关键组分GA20-oxidase氧化酶基因的研究进展北大核心CSCD

GA-20氧化酶(GA-20 oxidase)是重要的GA生物合成和调控酶,直接催化生成有生物活性的GAs,是一种多功能酶,最显著的特点就是负反馈调节。GA20-氧化酶在植物发育和生理过程中起着重要的调控作用。综述了高等植物体内GA20氧化酶基因的克隆及表达调控研究及其对株高、纤维、开花、产量性状等影响,重点阐述了GA20氧化酶基因与激素、光周期、抗性等之间的相互作用,以便更好地揭示GA-20氧化酶信号网络系统及其作用机制。     

高等植物赤霉素生物合成关键组分GA20-oxidase氧化酶基因的研究进展

GA-20氧化酶(GA-20 oxidase)是重要的GA生物合成和调控酶,直接催化生成有生物活性的GAs,是一种多功能酶,最显著的特点就是负反馈调节。GA20-氧化酶在植物发育和生理过程中起着重要的调控作用。综述了高等植物体内GA20氧化酶基因的克隆及表达调控研究及其对株高、纤维、开花、产量性状等影响,重点阐述了GA20氧化酶基因与激素、光周期、抗性等之间的相互作用,以便更好地揭示GA-20氧化酶信号网络系统及其作用机制。     

赤霉素生物合成与信号传递对植物株高的调控

植物株高是影响作物产量和品质的重要农艺性状。赤霉素(Gibberellins,GAs)是调控植物株高的重要激素,GA相关株高基因的克隆与分子机制研究对于合理调控作物生长发育和农业生产具有极其重要的利用价值,在水稻、小麦等粮食作物育种中得到了广泛应用。为了促进GA在果树、花卉等园艺作物育种中的有效利用,文中在分子生物学水平上介绍GA生物合成和GA信号传递途径对植物株高的调控。     

植物肌醇半乳糖苷合酶的生理功能和调控机制

植物肌醇半乳糖苷合酶（galactinol synthase, GolS）是高等植物棉子糖类寡糖合成途径中的关键酶,为棉子糖系列寡糖提供活化的半乳糖基,调控植物体内棉子糖（raffinose, RFO）系列寡糖的生物合成与积累。编码该酶的基因属于糖基转移酶（glycosyltransferases, GTs）GT8基因家族的亚家族。GolS参与合成的最终产物棉子糖家族低聚糖（raffinose family oligosaccharides,RFOs）是植物中重要的碳水化合物存在形式,在细胞内可溶性强,可作为脱水保护剂;还能发挥稳定膜结构的作用。同时,GolS催化合成的直接产物肌醇半乳糖苷（galactinol）和RFOs都能作为羟基自由基捕获分子参与活性氧的清除。因此,GolS参与的代谢途径在植物碳同化物的贮存与运输、生物和非生物逆境响应、种子的脱水效应等生命过程中均发挥了重要作用。GolS基因结构差异与表达模式不同,导致不同GolS基因参与的生物学功能具有很大的差异。研究植物中不同GolS基因的结构特征,组织特异性表达特性及它们响应不同生长发育阶段、环境变化的表达特性,对了解GolS参与的生物学功能具有重要意义。同时,在分子生物学水平上,深入了解调控植物GolS基因的分子调控机制,为通过遗传工程或分子辅助育种等手段,利用GolS改良农林作物的经济性状提供理论支持。本文针对近年来植物中GolS基因的生理功能和调控机制的研究进行了综述。     

植物肌醇半乳糖苷合酶的生理功能和调控机制

植物肌醇半乳糖苷合酶（galactinol synthase, GolS）是高等植物棉子糖类寡糖合成途径中的关键酶,为棉子糖系列寡糖提供活化的半乳糖基,调控植物体内棉子糖（raffinose, RFO）系列寡糖的生物合成与积累。编码该酶的基因属于糖基转移酶（glycosyltransferases, GTs）GT8基因家族的亚家族。GolS参与合成的最终产物棉子糖家族低聚糖（raffinose family oligosaccharides,RFOs）是植物中重要的碳水化合物存在形式,在细胞内可溶性强,可作为脱水保护剂;还能发挥稳定膜结构的作用。同时,GolS催化合成的直接产物肌醇半乳糖苷（galactinol）和RFOs都能作为羟基自由基捕获分子参与活性氧的清除。因此,GolS参与的代谢途径在植物碳同化物的贮存与运输、生物和非生物逆境响应、种子的脱水效应等生命过程中均发挥了重要作用。GolS基因结构差异与表达模式不同,导致不同GolS基因参与的生物学功能具有很大的差异。研究植物中不同GolS基因的结构特征,组织特异性表达特性及它们响应不同生长发育阶段、环境变化的表达特性,对了解GolS参与的生物学功能具有重要意义。同时,在分子生物学水平上,深入了解调控植物GolS基因的分子调控机制,为通过遗传工程或分子辅助育种等手段,利用GolS改良农林作物的经济性状提供理论支持。本文针对近年来植物中GolS基因的生理功能和调控机制的研究进行了综述。     

多效唑在植物组织培养中的应用

多效唑是英国ICI有限公司,在２０世纪８０年代末,推出的一种高效低毒的植物生长延缓剂。它通过阻碍贝壳杉烯向异贝壳杉烯酸的氧化,抑制生物体内赤霉素的生物合成,从而抑制植物的生长。目前在果树、蔬菜、花卉及大田粮食作物上已得到广泛应用。近年来,多效唑又开始在植物组织培养中应用,并取得了一定的效果。以下是多效唑在各种农作物和花卉组培中的应用效果简介,以供广大读者参考。一、在主要粮食作物上的应用：１．当多效唑加入到小麦花粉愈伤诱导及分化培养基中,对其出愈率及绿苗的分化率均影响不明显。而３mg／L的多效唑,对小…     

Effects of a Plant-Growth Regulator, Prohexadione, on the Biosynthesis of Gibberellins in Cell-Free Systems Derived from Immature Seeds

Inhibition of the biosynthesis of gibberellins by prohexadione,3,5-dioxo-4-propionylcyclo-hexanecarboxylic acid, was studiedwith cell-free systems derived from immature seeds of Cucur-bitamaxima, Phaseolus vulgaris and Pisum sativum. Prohexadione,at a concentration of 10–⁴ M, inhibited C-7 oxidationof GA₁₂-aldehyde, C-20 oxidation of GA₁₅, conversion of C₂₀-gib-berellinsto C₁₉-gibberellins, 3ß-hydroxylation, 2,3-dehydrogenationof GA²⁰, 2,3-epoxidation of GA₅ and 2ß-hydroxylationof GA₉ and GA₂₀. The 3ß-hydroxylase activity appearedto be more sensitive to prohexadione than were the C-20 oxygenaseand the 2ß-hydroxylase activities. The conversionof mevalonic acid to GA₁₂-aldehyde and the 13-hydroxylationof GA₁₂ were not affected by prohexadione at a concentrationof 3 ? 10^–4 M. All of the steps inhibited by prohexadioneare oxidation steps catalyzed by soluble enzymes that require2-oxoglutarate, Fe²⁺ and oxygen, and all of them occur distalto the synthesis of GA₁₂-aldehyde in the biosynthesis of gibberellins. (Received April 4, 1990; Accepted September 14, 1990)     

Potential sites of bioactive gibberellin production during reproductive growth in Arabidopsis

Gibberellin 3-oxidase (GA3ox) catalyzes the final step in the synthesis of bioactive gibberellins (GAs). We examined the expression patterns of all four GA3ox genes in Arabidopsis thaliana by promoter-beta-glucuronidase gene fusions and by quantitative RT-PCR and defined their physiological roles by characterizing single, double, and triple mutants. In developing flowers, GA3ox genes are only expressed in stamen filaments, anthers, and flower receptacles. Mutant plants that lack both GA3ox1 and GA3ox3 functions displayed stamen and petal defects, indicating that these two genes are important for GA production in the flower. Our data suggest that de novo synthesis of active GAs is necessary for stamen development in early flowers and that bioactive GAs made in the stamens and/or flower receptacles are transported to petals to promote their growth. In developing siliques, GA3ox1 is mainly expressed in the replums, funiculi, and the silique receptacles, whereas the other GA3ox genes are only expressed in developing seeds. Active GAs appear to be transported from the seed endosperm to the surrounding maternal tissues where they promote growth. The immediate upregulation of GA3ox1 and GA3ox4 after anthesis suggests that pollination and/or fertilization is a prerequisite for de novo GA biosynthesis in fruit, which in turn promotes initial elongation of the silique.     

Gibberellin Biosynthesis in Plants and Fungi: A Case of Convergent Evolution?

As well as being phytohormones, gibberellins (GAs) are present in some fungi and bacteria. Indeed, GAs were first discovered in the fungus Gibberella fujikuroi, from which gibberellic acid (GA3) and other GAs are produced commercially. Although higher plants and the fungus produce structurally identical GAs, there are important differences in the pathways and enzymes involved. This has become particularly apparent with the identification of almost all of the genes for GA-biosynthesis in Arabidopsis thaliana and G. fujikuroi, following the sequencing of the Arabidopsis genome and the detection of a GA-biosynthesis gene cluster in the fungus. For example, 3b-hydroxylation occurs early in the pathway in G. fujikuroi and is catalyzed by a cytochrome P450 monooxygenase, whereas it is usually the final step in plants and is catalyzed by 2-oxoglutarate-dependent dioxygenases. Similarly, 20-oxidation is catalyzed by dioxygenases in plants and a cytochrome P450 in the fungus. Even where cytochrome P450s have equivalent functions in plants and Gibberella, they are unrelated in terms of amino acid sequence. These profound differences indicate that higher plants and fungi have evolved their complex biosynthetic pathways to GAs independently and not by horizontal gene transfer.     

Gene-specific involvement of beta-oxidation in wound-activated responses in Arabidopsis

The coordinated induced expression of beta-oxidation genes is essential to provide the energy supply for germination and postgerminative development. However, very little is known about other functions of beta-oxidation in nonreserve organs. We have identified a gene-specific pattern of induced beta-oxidation gene expression in wounded leaves of Arabidopsis. Mechanical damage triggered the local and systemic induction of only ACX1 among acyl-coenzyme A oxidase (ACX) genes, and KAT2/PED1 among 3-ketoacyl-coenzyme A thiolase (KAT) genes in Arabidopsis. In turn, wounding induced KAT5/PKT2 only systemically. Although most of the beta-oxidation genes were activated by wound-related factors such as dehydration and abscisic acid, jasmonic acid (JA) induced only ACX1 and KAT5. Reduced expression of ACX1 or KAT2 genes, in transgenic plants expressing their corresponding mRNAs in antisense orientation, correlated with defective wound-activated synthesis of JA and with reduced expression of JA-responsive genes. Induced expression of JA-responsive genes by exogenous application of JA was unaffected in those transgenic plants, suggesting that ACX1 and KAT2 play a major role in driving wound-activated responses by participating in the biosynthesis of JA in wounded Arabidopsis plants.     

The biosynthesis of 12α-hydroxylated gibberellins in a cell-free system from cucurbita maxima endosperm

A previously unknown pathway for the biosynthesis of 12α-hydroxylated gibberellins was found in a cell-free system from Cucurbita maxima endosperm. The microsome fraction converts the gibberellin precursor GA_12-aldehyde simultaneously to GA₁₂ and 12α-hydroxy-GA₁₂-aldehyde. The ratio of these products is pH-dependent: above pH 6.5, the production of GA₁₂ is favoured, whilst below pH 6.5, 12α-hydroxy-GA₁₂-aldehyde is the predominant product. 12α-Hydroxy-GA₁₂-aldehyde is converted further by soluble enzymes to 12α-hydroxy-GA₁₄, 12α-hydroxy-GA₁₅, 12α-hydroxy-GA₃₇ and several unidentified products. This conversion is optimal between pH 6.0 and 6.5 in contrast to the previously known conversion of GA₁₂-aldehyde to GA₄₃ by soluble enzymes, which is optimal at pH 7.5. GA₅₈, a major 12α-hydroxylated endogenous constituent of C. maxima endosperm, was not obtained when 12α-hydroxy-GA₁₂-aldehyde was used as a substrate, but it was obtained together with GA₄ when GA₉ was incubated with a preparation containing both microsomal and soluble enzymes.     

Evolutionary diversification in polyamine biosynthesis

Polyamine biosynthesis is an ancient metabolic pathway present in all organisms. Aminopropyltransferases are key enzymes that mediate the synthesis of spermidine, spermine, and thermospermine. The relatively high sequence similarity between aminopropyltransferases and their similarity with putrescine N-methyltransferases (PMT) raises the question of whether they share a common ancestor or have evolved by convergence. Here we show that aminopropyltransferases and PMT are phylogenetically interconnected, and the different activities have been generated by unusually frequent events of diversification of existing functions. Although all spermidine synthases (SPDSs) derive from a common ancestor preceding the separation between prokaryotes and eukaryotes, they have been the origin of a variety of new activities. Among those, spermine synthases (SPMSs) represent a novelty independently arisen at least 3 times, in animals, fungi, and plants. The most parsimonious mechanism would involve the duplication and change of function of preexisting SPDS genes in each phylum. Although spermine is not essential for life, the repeated invention of SPMS and its conservation strongly argues for an evolutionary advantage derived from its presence. Moreover, the appearance of thermospermine synthase (tSPMS) in several genera of Archaea and Bacteria was accompanied by a loss of SPDS, suggesting that the new activity originated as a change of function of this enzyme. Surprisingly, tSPMS was later acquired by plants at an early stage of evolution by horizontal gene transfer and has proven to be essential for vascular development in tracheophytes. Finally, the synthesis of nicotine and tropane alkaloids in Solanales was favored by the origination of a new activity, PMT, as a duplication and change of function from SPDS.     

Pectins: structure, biosynthesis, and oligogalacturonide-related signaling.

Pectin is a family of complex polysaccharides present in all plant primary cell walls. The complicated structure of the pectic polysaccharides, and the retention by plants of the large number of genes required to synthesize pectin, suggests that pectins have multiple functions in plant growth and development. In this review we summarize the current level of understanding of pectin primary and tertiary structure, and describe new methods that may be useful to study localized pectin structure in the plant cell wall. We also discuss progress in our understanding of how pectin is biosynthesized and review the biological activities and possible modes of action of pectic oligosaccharides referred to as oligogalacturonides. We present our view of critical questions regarding pectin structure, biosynthesis, and function that need to be addressed in the coming decade. As the plant community works towards understanding the functions of the tens of thousands of genes expressed by plants, a large number of those genes are likely to be involved in the synthesis, turnover, biological activity, and restructuring of pectin. A combination of genetic, molecular, biochemical and chemical approaches will be necessary to fully understand the function and biosynthesis of pectin.