290 resultados para Auxin
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实验室前期工作证明OsRAA1在玉米泛素启动子驱动下组成型表达,可以抑制水稻初生根的生长,促进不定根的形成,形成不同程度螺旋状的初生根,根的向地性反应减缓,这些表型和野生型水稻用生长素处理的表型类似,而且OsRAA1基因的转录受生长素诱导,这些结果表明OsRAA1可能参与了生长素的信号转导途径。但这些表型产生的机理还不是很清楚。在水稻中,茉莉酸在根发育过程中的作用多为生理实验的报道;拟南芥中的研究表明生长素信号转导和茉莉酸信号转导可能都受26S蛋白酶体的调控。由此我们推测茉莉酸在根的发育过程中可能也起着同样的促进作用。本论文在超表达OsRAA1水稻基础上旨在克隆新基因,并对新基因功能进行研究,以探讨茉莉酸在水稻根发育过程中的分子机理,并对生长素和茉莉酸信号转导的关系进行探讨。 首先运用双向电泳技术结合质谱分析技术,在超表达OsRAA1水稻背景下发现了受体激酶家族DUF26的一个成员明显下调,我们命名为OsRMC(Oryza sativa Root Meander and Curling,AAL87185),Western杂交进一步证明了这个结果。 OsRMC位于4号染色体,信息学分析表明只有一个拷贝,没有内含子,ORF阅读框为777bp,编码的蛋白分子量为27.9 kDa,等电点(pI)为5.01。对该蛋白进行同源性比较发现,其含有2个C-X8-C-X2-C基序(Cys-rich repeat, CRR)即半胱氨酸富集区,其中第四个半胱氨酸残基不保守,该基序会形成二硫键,编码两个未知功能的DUF26(Domain Unknown Function 26)结构域。OsRMC由一个信号肽和两个CRR区组成,但没有跨膜区和激酶区。RT-PCR显示OsRMC可能是组成型表达的基因;亚细胞实验表明OsRMC是膜定位的蛋白。Western blot显示OsRMC受茉莉酸诱导表达,受生长素的抑制。 RNAiOsRMC转基因水稻在暗处培养时,抑制了初生根的生长,使侧根数目减少,但促进了不定根的生长和数目的增加;第二叶鞘变短,这些表型和前人报道的外源茉莉酸处理野生型的表型一致。转基因对生长素信号转导和合成没有影响,但初生根和第二叶鞘对外源茉莉酸更加敏感,说明RNAiOsRMC转基因水稻可能增强了茉莉酸信号转导途径。分析转基因水稻的茉莉酸信号转导途径部分相关基因的表达变化,根中受茉莉酸信号转导特异诱导的病原相关基因RSOsPR10的表达明显增多,而JAmyb和OsNDPK1的表达没有变化,证实转基因增强了茉莉酸信号转导其中的一个路径;进一步分析茉莉酸合成途径12-OXO-PDA(12-氧代-顺,顺-10,15-植物二烯酸)还原酶基因OsOPR的表达发现与野生型没有明显差别,说明转基因可能没有影响体内的茉莉酸合成途径。RNAiOsRMC转基因水稻的初生根比野生型的更容易发生弯曲,实验表明培养过程中茉莉酸和背触反应(negative thigmotropism)共同作用使转基因的初生根更容易发生卷曲,而光信号会增强卷曲程度。但RNAiOsRMC转基因水稻并没有影响根的向地性,暗示RNAiOsRMC转基因可能增强了根的回旋运动或(和)背触反应,从而促进了根的弯曲和卷曲。这些结果证明OsRMC参与的茉莉酸信号转导过程在水稻根的发育、弯曲和卷曲过程中起着重要的促进作用。通过对超表达OsRAA1和RNAiOsRMC转基因水稻的分析,说明水稻中存在着生长素信号转导促进茉莉酸信号转导的途径。 综合以上实验结果认为,OsRAA1调控了受体激酶家族DUF26的一个成员OsRMC,使其表达量降低,该过程增强了茉莉酸信号转导途径;确认了受体激酶家族DUF26的基因具有重要的生物学功能,证实了OsRMC调控的茉莉酸信号转导在水稻根系发育、根弯曲和卷曲过程中具有重要的促进作用;证明水稻中存在着生长素信号转导促进茉莉酸信号转导的途径,为完善各种植物激素调控水稻根系发育的网络提供了新的实验证据。
Resumo:
SKP1 (S-phase kinase-associated-protein 1) 家族蛋白是普遍存在于真核生物中的一类小分子量蛋白质,其主要的生物学功能在于参与SCF复合体的形成,从而调控生物体内泛素介导的蛋白质降解,并参与多方面的生物发育过程。SKP1蛋白能够同时和Cullin蛋白以及F-box蛋白结合,形成SCF复合体的核心部分。因此,SKP1正常功能的维持对于SCF复合体功能的实现至关重要。研究显示,植物中尤其是以拟南芥为代表模式植物中已经发现了21个SKP1基因成员,并发现其中的ASK1参与了多个SCF复合体的形成并调控着包括植物雄性减数分裂、生长素、赤霉素、茉莉酸和乙烯等生理和发育进程。但是来自高等植物尤其是小麦和水稻中的SKP1基因还鲜有报道,其功能还不为所知;此外,SKP1基因与ABA的关系还没有任何报道。 本文利用筛选小麦减数分裂期小花的cDNA文库结合RT-PCR的方法从小麦中分离到了一个SKP1同源基因,并命名为TSK1 (Triticum aestivum SKP1-Like 1)。序列比较结果显示TSK1与多个植物来源的SKP1基因有较高的同源性,对其推测的编码蛋白序列的分析发现TSK1与包括拟南芥来源的ASK1/ASK2等蛋白的羧基端存在非常高的保守性。 在对TSK1表达模式的研究中,本文发现TSK1主要是集中在小麦花序和幼根中表达。利用多种激素对小麦幼苗处理之后,发现TSK1的表达受ABA的抑制,但是当小麦中ABA合成受抑的情况下,TSK1的表达会有所增加,说明TSK1的表达受ABA的调控。RNA原位杂交显示TSK1基因在花顶端分生组织、花药以及幼根等分生较旺盛的组织中有较强的表达,暗示该基因可能参与了与细胞分裂相关的过程。 为了研究TSK1可能具有的功能,本文首先在ask1-1突变体背景上超表达TSK1,发现能够部分恢复ask1-1突变体雄性不育的表型,说明TSK1和ASK1在植物减数分裂过程中存在某种保守性。 在野生型拟南芥中超表达TSK1造成了拟南芥多个方面的变化,包括萌发和开花推迟,气孔开度减小等。进一步的观察发现,转基因植株的萌发和营养生长都呈现出对ABA的超敏感,后续证据证实这种ABA的超敏感性并不是由于转基因拟南芥中ABA合成途径的改变所造成的,而极有可能是影响了ABA的信号传导过程。RT-PCR的结果显示,转基因植株中多个ABA相关的已知基因表达量的发生了变化。 为了提供植物中SKP1家族成员参与调节植物ABA信号传导途径证据,本文对拟南芥ASK1/ask1 ASK12/ask2的杂合双突变体自交后代进行了研究。结果显示,ask1/ask1纯合突变体和ask1/ask1 ASK2/ask2植株表现出对ABA的弱敏感性。该结果从另一个侧面印证了TSK1超表达植株对ABA超敏感表型。 此外,TSK1超表达拟南芥也表现出生长素相关表型,也印证了该基因可能与ASK1类似,参与到生长素介导的根发育过程。 综上所述,本文认为TSK1参与了植物激素介导的植物发育过程,而且极有可能是形成了目前未知的某种SCF复合体。最重要的是,本文的结果为SCF复合体参与调节植物ABA信号传导途径提供了生理及遗传层面的证据。
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本论文以显花植物水稻和拟南芥为对象,研究植物器官形成激素调控的分子机理。发现拟南芥干细胞决定基因WUS和ABA信号关键调节因子ABI3间存在相互调节关系,它们对质体和根毛发育等具有调控作用;运用细胞学手段对OsAGAP和OsRMC调控根发育的机理进行了研究。这些结果为了解ABA、生长素和JA等激素对分生组织或根等器官的形成的调控机理提供了新资料。 拟南芥WUS基因是一个重要的干细胞决定基因。在茎尖分生组织和花分生组织的动态平衡调节中各存在一个反馈调节环:WUS促进CLV3的表达,而CLV3 反馈抑制WUS表达,它们共同决定干细胞的数目;在WUS+LFY 和AG之间也存在一个类似的反馈环,负责花器官的正常启动和终止。本工作发现在外源ABA 存在下,拟南芥WUS功能获得突变体sef (stem ectopic flowers)子叶黄化过程受到抑制,即sef突变体对ABA 的敏感性降低,而且在sef突变体中ABI3转录水平下调,说明WUS 抑制ABI3的表达。另一方面,在abi3突变体中WUS转录水平下降,启动子分析发现WUS是ABI3所在的B3结构域家族基因的靶基因,酵母单杂交实验表明B3家族蛋白FUS3可以与WUS调控区结合;外源ABA 处理pWUS::GUS植株发现ABA可使WUS异位表达,暗示受ABA信号诱导的B3类转录因子可与WUS调控区结合,从而促进WUS的表达。这些结果支持ABI3/WUS间的反馈调节机理,该调节环可能参与调控拟南芥质体和根毛发育等过程。 双子叶和单子叶植物的发育和器官形成高度依赖生长素极性运输(PAT), 生长素输入和输出载体的准确定位对于极性运输的正常进行是必要的。在双子叶模式植物拟南芥中,生长素输出载体PIN1的转运和定位受小G蛋白ARF鸟苷酸转换因子GNOM介导。本实验室克隆到一个水稻ARF GAPase激活蛋白OsAGAP, 其超表达引起PAT改变且干扰主根和侧根的发生及发育。前期生理实验显示超表达植株侧根的表型可被膜渗透性生长素NAA恢复,但不能被载体依赖型生长素IAA和2, 4-D恢复。为了解释OsAGAP过表达引起根系发育受到抑制的表型,本工作主要从细胞学角度继续深入分析OsAGAP介导生长素运输的机理。实验发现,OsAGAP超表达植株中AUX1在细胞中分布改变;生长素输出载体PIN1和PIN2的定位不受影响;该基因的超表达使囊泡聚集,形成类似囊泡运输抑制剂BFA处理后的结构;OsAGAP与细胞转运系统中的高尔基体存在部分共定位。以上结果表明OsAGAP调节小G蛋白Arf的活性,参与调控生长素极性运输过程,进而调控根系发育。通过对JA诱导的OsRMC蛋白的膜定位分析及转基因植株根中JA合成水平的测定,为研究此蛋白参与JA信号、调控根系发育提供了直接证据。 此外,论文还对拟南芥STAR2基因的功能进行了一定的初探。
Resumo:
植物根系大小和形态是决定植物吸氮能力的重要因素,而植物根系生长发育与土壤中营养元素的分布及其有效性密切相关,尤其是硝酸盐。然而目前关于硝酸盐调节植物根系生长的生理机制仍不清楚。一氧化氮(NO)是一种重要的气体信号分子,参与植物体内多种生理生化过程,包括调节根的生长发育。本研究以玉米自交系478为材料,采用营养液培养法,探讨了NO在硝酸盐调节玉米根系生长中的作用。主要结果和结论如下: 玉米幼苗在不同硝酸盐水平下生长7天后,主根伸长随着硝酸盐浓度的升高而下降;与0.01 mM硝酸盐处理下的玉米主根伸长相比,0.1 mM和1 mM硝酸盐处理对玉米主根伸长分别抑制了30%和36%。随着硝酸盐浓度的增加,玉米主根根尖过氧化氢(H2O2)含量表现出降低的趋势,而抗氧化酶,如超氧化物歧化酶(SOD)、过氧化氢酶(CAT)、过氧化物酶(POD)的活性则表现出增加的趋势。外源供应过氧化氢对低浓度硝酸盐(0.01 mM)和高浓度硝酸盐(10 mM)处理下的玉米根伸长都没有影响,这表明了根尖过氧化氢含量的下降不是高浓度硝酸盐抑制玉米主根伸长的原因。 NO供体硝普钠(SNP)能够缓解高浓度硝酸盐对玉米主根伸长的抑制,而对低浓度硝酸盐处理下的主根伸长没有影响,而且NO清除剂亚甲基兰(MB)和NO合成酶抑制剂Nω-硝基-L-精氨酸(L-NNA)显著抑制了低浓度硝酸盐处理下的玉米主根伸长,而对高浓度硝酸盐处理下的玉米主根伸长没有影响。用NO特异性荧光染料4,5-二氨基乙酰乙酸荧光素(DAF-2DA)检测结果表明:高浓度硝酸盐显著降低玉米根尖NO含量。而玉米根中的硝酸还原酶活性随硝酸盐浓度的增加而增加。以上结果说明,高浓度硝酸盐抑制玉米主根伸长可能是与根尖NO合成酶的下调所导致的内源NO含量的降低有关。 另外,外源生长素(IAA)能缓解高浓度硝酸盐对玉米主根伸长的抑制,同时,也增加了高浓度硝酸盐处理下玉米根中内源NO含量,而对低浓度硝酸盐处理下的玉米根中内源NO没有影响。因此推测,根尖生长素的下降导致内源NO含量的降低可能是高浓度硝酸盐抑制玉米主根伸长的原因。
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Vesicle trafficking plays an important role in cell division, establishment of cell polarity, and translation of environmental cues to developmental responses. However, the molecular mechanisms regulating vesicle trafficking remain poorly understood. Here, we report that the evolutionarily conserved caspase-related protease separase (EXTRA SPINDLE POLES [ESP]) is required for the establishment of cell polarity and cytokinesis in Arabidopsis thaliana. At the cellular level, separase colocalizes with microtubules and RabA2a (for RAS GENES FROM RAT BRAINA2a) GTPase-positive structures. Separase facilitates polar targeting of the auxin efflux carrier PIN-FORMED2 (PIN2) to the rootward side of the root cortex cells. Plants with the radially swollen4 (rsw4) allele with compromised separase activity, in addition to mitotic failure, display isotropic cell growth, perturbation of auxin gradient formation, slower gravitropic response in roots, and cytokinetic failure. Measurements of the dynamics of vesicle markers on the cell plate revealed an overall reduction of the delivery rates of KNOLLE and RabA2a GTPase in separase-deficient roots. Furthermore, dissociation of the clathrin light chain, a protein that plays major role in the formation of coated vesicles, was slower in rsw4 than in the control. Our results demonstrate that separase is a key regulator of vesicle trafficking, which is indispensable for cytokinesis and the establishment of cell polarity.
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The aims of this work were to deepen the knowledge on the physiology of bract abscission in Bougainvillea spectabilis ‘Killie Campbell’ plants, in what relates to respiration and carbon balance. Using the effects induced by Silver Thiosulphate (STS) and/or Naphtalene Acetic Acid (NAA, at high concentration: 500 mg.l-1) on bract abscission under interior conditions, the relationship between bract survival time (longevity) and, respiration rate or carbohydrate levels, was investigated. Treatments that included NAA were the ones that reduced significantly bract abscission. Unexpectedly, the higher the levels of bract soluble and total carbohydrates, measured at day 10 postproduction (PP), the higher the abscission of bracts. These results show, for the first time, that abscission can positively correlate with non structural carbohydrates levels in the organ that abscise. Bract respiration rate was significantly affected by treatment and postproduction day (PP). Treatments that had higher bract respiration rates (WATER and STS) also had higher levels of non structural carbohydrates in the bracts. Bract respiration rate decreased from day 10 to day 17 PP by approximately 50% (on average of all treatments) and was negatively correlated with bract survival time. In the carbon balance per gram of bract dry weight, the treatments WATER and STS, showed the largest decrease in the content of total carbohydrates and had the highest consumption of carbohydrates through respiration. So, these were the bracts that needed to import a higher amount of carbohydrates per gram of bract dry weight. In the carbon balance for the whole mass of bracts and adjacent stems in an average plant, the treatments WATER and STS continued to allow for the largest decreases in total carbohydrate during postproduction. However, and contradicting the results per gram of bract dry weight, the highest total consumption of carbohydrates by respiration was obtained for the NAA and STS+NAA treatments. It makes sense that bracts that last longer have lower individual carbon consumption while, at the plant level, the increased number of remaining bracts causes a higher overall expenditure. Respiration rate has been used as an indicator of flower longevity, this correlation is here extended for the flower+bract system. Plants that had higher bract respiration rates, most probably, had a higher flow of carbohydrates through the bracts (and flowers), which, in the end, was sensed as a higher carbohydrate level.
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The cell cycle comprise the four phases of, G1, S-phase, G2 and mitosis. Two critical transitions are G1/S and G2/M; the latter is regulated by WEE1 kinase and CDC25 phosphatases. The scope of this thesis was to investigate the regulation of the G2/M transition of the cell cycle by WEE1 and CDC25, and how these genes interface with plant growth regulators in Arabidopsis thaliana. In Arabidopsis roots, the frequency of lateral roots was found to be increased by ectopic expression of Schizosaccharomyces pombe (Sp)cdc25e and reduced by Arath;WEE1 expression. I examined the effect of Arath;WEE1 and Spcdc25 on induction of shoots and roots in Arabidopsis hypocotyls in vitro. Hypocotyl explants from two over-expressing WEE1 lines , three T-DNA insertion lines and two expressing cdc25 (Spcdc25e) lines together with wild type (WT) were cultured on two-way gradients of kinetin (Kin) and naphthyl acetic acid (NAA). Below a threshold concentration of NAA (100 ng ml-1), WEE1 repressed morphogenesis in vitro, whereas at all NAA/Kin combinations Spcdc25 promoted morphogenesis (particularly root formation) over and above that in WT. Loss of function wee1-1 cultures were very similar to WT. Quantitative data indicated a significant increase in the frequency of root formation in Spcdc25e cultures compared with WT particularly at low Kin concentrations, and WEE1oe’s repressive effect was overcome by NAA but not Kin. In conclusion, WEE1 has a repressive effect on morphogenesis in vitro that can be overcome by auxin whereas Spcd25 by-passes a cytokinin requirement for the induction of morphogenesis in vitro. The role of CDC25 and WEE1 in DNA damage responses was also analysed. Two over-expressing Arath;CDC25 lines and T-DNA mutants showed no difference to WT either in standard conditions or zeocin-supplemented treatments. However, root length was longer in Arath;CDC25oe lines treated with hydroxyurea (HU) and lateral root number was increased compared to WT. This suggests a differential response of Arath;CDC25oe in the DNA replication (HU-induced) and DNA damage (zeocin-induced) checkpoints (Chapter 5). Finally the roles of WEE1 and CDC25 in cell cycle regulation were examined using tobacco TBY-2 cell cultures expressing Arath;WEE1, Nicotiana tabacum (Nicta)WEE1 or Arath;CDC25. Whilst Nicta;WEE1 lengthened G2 of the cell cycle, Arath;WEE1 had an unusual effect of shortening G2 phase and Arath;CDC25 had no observable effect (Chapter 6).
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Background Entry into mitosis is regulated by cyclin dependent kinases that in turn are phosphoregulated. In most eukaryotes, phosphoregulation is through WEE1 kinase and CDC25 phosphatase. In higher plants a homologous CDC25 gene is unconfirmed and hence the mitotic inducer Schizosaccharomyces pombe (Sp) cdc25 has been used as a tool in transgenic plants to probe cell cycle function. Expression of Spcdc25 in tobacco BY-2 cells accelerates entry into mitosis and depletes cytokinins; in whole plants it stimulates lateral root production. Here we show, for the first time, that alterations to cytokinin and ethylene signaling explain the rooting phenotype elicited by Spcdc25 expression in Arabidopsis. Results Expressing Spcdc25 in Arabidopsis results in increased formation of lateral and adventitious roots, a reduction of primary root width and more isodiametric cells in the root apical meristem (RAM) compared with wild type. Furthermore it stimulates root morphogenesis from hypocotyls when cultured on two way grids of increasing auxin and cytokinin concentrations. Microarray analysis of seedling roots expressing Spcdc25 reveals that expression of 167 genes is changed by > 2-fold. As well as genes related to stress responses and defence, these include 19 genes related to transcriptional regulation and signaling. Amongst these was the up-regulation of genes associated with ethylene synthesis and signaling. Seedlings expressing Spcdc25 produced 2-fold more ethylene than WT and exhibited a significant reduction in hypocotyl length both in darkness or when exposed to 10 ppm ethylene. Furthermore in Spcdc25 expressing plants, the cytokinin receptor AHK3 was down-regulated, and endogenous levels of iPA were reduced whereas endogeous IAA concentrations in the roots increased. Conclusions We suggest that the reduction in root width and change to a more isodiametric cell phenotype in the RAM in Spcdc25 expressing plants is a response to ethylene over-production. The increased rooting phenotype in Spcdc25 expressing plants is due to an increase in the ratio of endogenous auxin to cytokinin that is known to stimulate an increased rate of lateral root production. Overall, our data reveal important cross talk between cell division and plant growth regulators leading to developmental changes.
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In Arabidopsis (Arabidopsis thaliana), the blue light photoreceptor phototropins (phot1 and phot2) fine-tune the photosynthetic status of the plant by controlling several important adaptive processes in response to environmental light variations. These processes include stem and petiole phototropism (leaf positioning), leaf flattening, stomatal opening, and chloroplast movements. The PHYTOCHROME KINASE SUBSTRATE (PKS) protein family comprises four members in Arabidopsis (PKS1-PKS4). PKS1 is a novel phot1 signaling element during phototropism, as it interacts with phot1 and the important signaling element NONPHOTOTROPIC HYPOCOTYL3 (NPH3) and is required for normal phot1-mediated phototropism. In this study, we have analyzed more globally the role of three PKS members (PKS1, PKS2, and PKS4). Systematic analysis of mutants reveals that PKS2 (and to a lesser extent PKS1) act in the same subset of phototropin-controlled responses as NPH3, namely leaf flattening and positioning. PKS1, PKS2, and NPH3 coimmunoprecipitate with both phot1-green fluorescent protein and phot2-green fluorescent protein in leaf extracts. Genetic experiments position PKS2 within phot1 and phot2 pathways controlling leaf positioning and leaf flattening, respectively. NPH3 can act in both phot1 and phot2 pathways, and synergistic interactions observed between pks2 and nph3 mutants suggest complementary roles of PKS2 and NPH3 during phototropin signaling. Finally, several observations further suggest that PKS2 may regulate leaf flattening and positioning by controlling auxin homeostasis. Together with previous findings, our results indicate that the PKS proteins represent an important family of phototropin signaling proteins.
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Chez les angiospermes, la reproduction passe par la double fécondation. Le tube pollinique délivre deux cellules spermatiques au sein du gamétophyte femelle. Une cellule féconde la cellule œuf pour produire un zygote; l’autre féconde la cellule centrale pour produire l’endosperme. Pour assurer un succès reproductif, le développement du gamétophyte femelle au sein de l’ovule doit établir un patron cellulaire qui favorise les interactions avec le tube pollinique et les cellules spermatiques. Pour ce faire, un dialogue doit s’établir entre les différentes cellules de l’ovule lors de son développement, de même que lors de la fécondation. D’ailleurs, plusieurs types de communications intercellulaires sont supposées suite à la caractérisation de plusieurs mutants développementaux. De même, ces communications semblent persister au sein du zygote et de l’endosperme pour permettre la formation d’un embryon viable au sein de la graine. Malgré les développements récents qui ont permis de trouver des molécules de signalisation supportant les modèles d’interactions cellulaires avancés par la communauté scientifique, les voies de signalisation sont de loin très incomplètes. Dans le but de caractériser des gènes encodant des protéines de signalisation potentiellement impliqués dans la reproduction chez Solanum chacoense, l’analyse d’expression des gènes de type RALF présents dans une banque d’ESTs (Expressed Sequence Tags) spécifiques à l’ovule après fécondation a été entreprise. RALF, Rapid Alcalinization Factor, est un peptide de 5 kDa qui fait partie de la superfamille des «protéines riches en cystéines (CRPs)», dont les rôles physiologiques au sein de la plante sont multiples. Cette analyse d’expression a conduit à une analyse approfondie de ScRALF3, dont l’expression au sein de la plante se limite essentiellement à l’ovule. L’analyse de plantes transgéniques d’interférence pour le gène ScRALF3 a révélé un rôle particulier lors de la mégagamétogénèse. Les plantes transgéniques présentent des divisions mitotiques anormales qui empêchent le développement complet du sac embryonnaire. Le positionnement des noyaux, de même que la synchronisation des divisions au sein du syncytium, semblent responsables de cette perte de progression lors de la mégagamétogénèse. L’isolement du promoteur de même que l’analyse plus précise d’expression au sein de l’ovule révèle une localisation sporophytique du transcrit. La voie de signalisation de l’auxine régule également la transcription de ScRALF3. De surcroît, ScRALF3 est un peptide empruntant la voie de sécrétion médiée par le réticulum endoplasmique et l’appareil de Golgi. En somme, ScRALF3 est un important facteur facilitant la communication entre le sporophyte et le gamétophyte pour amener à maturité le sac embryonnaire. L’identification d’un orthologue potentiel chez Arabidopsis thaliana a conduit à la caractérisation de AtRALF34. L’absence de phénotype lors du développement du sac embryonnaire suggère, cependant, de la redondance génétique au sein de la grande famille des gènes de type RALF. Néanmoins, les peptides RALFs apparaissent comme d’importants régulateurs lors de la reproduction chez Solanum chacoense et Arabidopsis thaliana.
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Random genetic changes generated during in vitro culture are not desirable for plant micropropagation and genetic transformation. RAPD markers were used to detect the variation in leaf disc callus cultures of Jatropha curcas, maintained in Murashige and Skoog (MS) medium with different auxin and cytokinin combinations. In total 41 scorable bands were produced with 11 primers. Out of 41 bands, 37 were polymorphic (91.12%). The average number of polymorphic bands was 3.36 per primer. The highest similarity (0.82) with mother plant was seen in callus maintained on MS with hormonal combination Indole butyric acid - 0.4mg/l+ N6-benzyladenine purine - 4.0 mg/l. The callus grown on MS with hormonal combinations IBA- 0.4mg/l+ BAP- 2.0mg/l, IBA- 0.4mg/l+ BAP- 2.5mg/l and IBA- 0.6 mg/l+ BAP- 2.0 mg/l also showed similarity with the mother plant. Callus maintained on MS with hormonal combination IBA- 0.2mg/l+ BAP- 2.0 mg/l was found to show least similarity (0.53) with mother plant
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This review summarizes the recent discovery of the cupin superfamily (from the Latin term "cupa," a small barrel) of functionally diverse proteins that initially were limited to several higher plant proteins such as seed storage proteins, germin (an oxalate oxidase), germin-like proteins, and auxin-binding protein. Knowledge of the three-dimensional structure of two vicilins, seed proteins with a characteristic beta-barrel core, led to the identification of a small number of conserved residues and thence to the discovery of several microbial proteins which share these key amino acids. In particular, there is a highly conserved pattern of two histidine-containing motifs with a varied intermotif spacing. This cupin signature is found as a central component of many microbial proteins including certain types of phosphomannose isomerase, polyketide synthase, epimerase, and dioxygenase. In addition, the signature has been identified within the N-terminal effector domain in a subgroup of bacterial AraC transcription factors. As well as these single-domain cupins, this survey has identified other classes of two-domain bicupins including bacterial gentisate 1, 2-dioxygenases and 1-hydroxy-2-naphthoate dioxygenases, fungal oxalate decarboxylases, and legume sucrose-binding proteins. Cupin evolution is discussed from the perspective of the structure-function relationships, using data from the genomes of several prokaryotes, especially Bacillus subtilis. Many of these functions involve aspects of sugar metabolism and cell wall synthesis and are concerned with responses to abiotic stress such as heat, desiccation, or starvation. Particular emphasis is also given to the oxalate-degrading enzymes from microbes, their biological significance, and their value in a range of medical and other applications.
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Background: Maize is a good model system for cereal crop genetics and development because of its rich genetic heritage and well-characterized morphology. The sequencing of its genome is well advanced, and new technologies for efficient proteomic analysis are needed. Baculovirus expression systems have been used for the last twenty years to express in insect cells a wide variety of eukaryotic proteins that require complex folding or extensive posttranslational modification. More recently, baculovirus display technologies based on the expression of foreign sequences on the surface of Autographa californica ( AcMNPV) have been developed. We investigated the potential of a display methodology for a cDNA library of maize young seedlings. Results: We constructed a full-length cDNA library of young maize etiolated seedlings in the transfer vector pAcTMVSVG. The library contained a total of 2.5 x 10(5) independent clones. Expression of two known maize proteins, calreticulin and auxin binding protein (ABPI), was shown by western blot analysis of protein extracts from insect cells infected with the cDNA library. Display of the two proteins in infected insect cells was shown by selective biopanning using magnetic cell sorting and demonstrated proof of concept that the baculovirus maize cDNA display library could be used to identify and isolate proteins. Conclusion: The maize cDNA library constructed in this study relies on the novel technology of baculovirus display and is unique in currently published cDNA libraries. Produced to demonstrate proof of principle, it opens the way for the development of a eukaryotic in vivo display tool which would be ideally suited for rapid screening of the maize proteome for binding partners, such as proteins involved in hormone regulation or defence.
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The inability of a plant to grow roots rapidly upon transplanting is one of the main factors contributing to poor establishment. In bare-rooted trees, treatments such as root pruning or application of the plant hormone auxin [e.g., indole butyric acid (IBA)] can promote root growth and aid long-term establishment. There is little information on ornamental containerised plants, however, other than the anecdotal notion that 'teasing' the roots out of the rootsoil mass before transplanting can be beneficial. In the present study we tested the ability of various root-pruning treatments and application of IBA to encourage new root and shoot growth in two shrub species, commonly produced in containers - Buddleja davidii 'Summer Beauty' and Cistus 'Snow Fire'. In a number of experiments, young plants were exposed to root manipulation (teasing, light pruning, or two types of heavy pruning) and/or treatment with IBA (at 500 or 1,000 mg l-1) before being transplanted into larger containers containing a medium of 1:1:1 (v/v/v) fine bark, sand and loam. Leaf stomatal conductance (gl) was measured 20 min, and 1, 2, 4 and 6 h after root manipulation. Net leaf CO2 assimilation (A) was measured frequently during the first week after transplanting, then at regular intervals up to 8 weeks after transplanting. Plants were harvested 8 weeks after transplanting, and root and shoot weights were measured. In both species, light root pruning alone, or in combination with 500 mg l-1 IBA, was most effective in stimulating root growth. In contrast, teasing, which is commonly used, showed no positive effect on root growth in Buddleja, and decreased new root growth in Cistus. The requirement for exogenous auxin to encourage new root growth varied between experiments and appeared to be influenced by the age and developmental stage of the plants. There were no consistent responses between root treatments and net CO2 assimilation rates, and changes in root weight were not closely correlated with changes in assimilation. The mechanisms whereby new root growth is sustained are discussed.
