Functions For OsMADS2 And OsMADS1 As Master Regulators Of Gene Expression During Rice Floret Meristem Specification And Organ Development

Yadav, Shri Ram

09 1900

Plant reproductive development begins when vegetative shoot apical meristems change their fate to inflorescence meristems which develop floral meristems on the flanks. This process of meristem fate change and organ development involves regulated activation and/or repression of many cell fate determining factors that execute down-stream gene expression cascades. Flowers are formed when floral organs are specified on the floral meristem in four concentric whorls. In the model dicot plant Arabidopsis, the identity and pattern of floral organs is determined by combined actions of MADS-domain containing transcription factors of the classes A, B, C, D and E. Rice florets are produced on a compact higher order branch of the inflorescence and have morphologically distinct non-reproductive organs that are positioned peripheral to the male and female reproductive organs. These unique outer organs are the lemma and palea that create a closed floret internal to which are a pair of lodicules that are asymmetrically positioned fleshy and reduced petal-like organs. The unique morphology of these rice floret organs pose intriguing questions on how evolutionary conserved floral meristem specifying and organ fate determining factors bring about their distinct developmental functions in rice. We have studied the functions for two rice MADS-box proteins, OsMADS2 and OsMADS1, to understand their role as master regulators of gene expression during rice floret meristem specification and organ development. OsMADS2; a transcriptional regulator of genes expression required for lodicule development Arabidopsis B-function genes AP3 and PI are stably expressed in the whorl 2 and 3 organ primordia and they together with other MADS-factors (Class A+E or C+E) regulate the differentiation of petals and stamens (Jack et al, 1992; Goto and Meyerowitz, 1994). Rice has a single AP3 ortholog, SPW1 (OsMADS16) but has duplicated PI-like genes, OsMADS2 and OsMADS4. Prior studies in our lab on one of these rice PI-like genes OsMADS2 showed that it is needed for lodicule development but is dispensable for stamen specification (Kang et al., 1998; Prasad and Vijayraghavan, 2003). Functional divergence between OsMADS2 and OsMADS4 may arise from protein divergence or from differences in their expression patterns within lodicule and stamen whorls. In this study, we have examined the dynamic expression pattern of both rice PI-like genes and have examined the likelihood of their functional redundancy for lodicule development. We show OsMADS2 transcripts occur at high levels in developing lodicules and transcripts are at reduced levels in stamens. In fully differentiated lodicules, OsMADS2 transcripts are more abundant in the distal and peripheral regions of lodicules, which are the tissues that are severely affected in OsMADS2 knock-down florets (Prasad and Vijayraghavan, 2003). The onset of OsMADS4 expression is in very young floret meristems before organ primordia emergence and this is expressed before OsMADS2. In florets undergoing organogenesis, high level OsMADS4 expression occurs in stamens and carpels and transcripts are at low level in lodicules (Yadav, Prasad and Vijayraghvan, 2007). Thus, we show that these paralogous genes differ in the onset of their activation and their stable transcript distribution within lodicules and stamens that are the conserved expression domains for PI-like genes. Since the expression of OsMADS4 in OsMADS2 knock-down florets is normal, our results show OsMADS2 has unique functions in lodicule development. Thus our data show subfunctionalization of these paralogous rice PI-like genes. To identify target genes regulated by OsMADS2 that could contribute to lodicule differentiation, we have adopted whole genome transcript analysis of wild-type and dsRNAiOsMADS2 panicles with developing florets. This analysis has identified potential down-stream targets of OsMADS2 many of which encode transcription factors, components of cell division cycle and signalling factors whose activities likely control lodicule differentiation. The expression levels of few candidate targets of OsMADS2 were examined in various floret organs. Further, the spatial expression pattern for four of these down-stream targets of OsMADS2 was analysed and we find overlap with OsMADS2 expression domains (Yadav, Prasad and Vijayraghvan, 2007). The predicted functions of these OsMADS2 target genes can explain the regulation of growth and unique vascular differentiation of this short fleshy modified petal analog. OsMADS1, a rice E-class gene, is a master regulator of other transcription factors and auxin and cytokinin signalling pathways In Arabidopsis four redundant SEPALLATA factors (E-class) are co-activators of other floral organ fate determining MADS-domain factors (classes ABCD) and thus contribute to floral meristem and floral organ development (Krizek and Fletcher, 2005). Among the grass-specific sub-clade of SEP-like genes, rice OsMADS1 is the best characterized. Prior studies in our lab showed that OsMADS1 is expressed early throughout the floret meristem before organ primordia emergence and later is restricted to the developing lemma and palea primordia with weak expression in carpel (Prasad et al, 2001). Stable expression continues in these floret organs. OsMADS1 plays critical non-redundant functions to specify a determinate floret meristem and also regulates floret organ identities (Jeon et al., 2000; Prasad et al, 2001; 2005; Agarwal et al., 2005; Chen et al., 2006). In the present study, we have adopted two different functional genomic approaches to identify genes down-stream of OsMADS1 in order to understand its mechanism of action during floret development. We have studied global transcript profiles in WT and dsRNAiOsMADS1 panicles and find OsMADS1 is a master regulator of a significant fraction of the genome’s transcription factors and also a number of genes involved in hormone-dependent cell signalling. We have validated few representative genes for transcription factors as targets regulated by OsMADS1. In a complementary approach, we have determined the consequences of induced-ectopic over-expression of a OsMADS1:ΔGR fusion protein in shoot apical meristems of transgenic plants. Transcript levels for candidate target genes were assessed in induced tissues and compared to mock-treated meristems and also with meristems induced for OsMADS1:ΔGR but blocked for new protein synthesis. These analyses show that OsMADS55 expression is directly regulated by OsMADS1. Importantly, OsMADS55 is related to SVP that plays an important role in floral transition and floral meristem identity in Arabidopsis. OsHB3 and OsHB4, homeodomain transcription factors, with a probable role in meristem function, are also directly regulated by OsMADS1. The regulation of such genes by OsMADS1 can explain its role in floret meristem specification. In addition to regulating other transcription factors, OsMADS1 knock-down affects expression of genes encoding proteins in various steps of auxin and cytokinin signalling pathways. Our differential expression profiling showed OsMADS1 positively regulates the auxin signalling pathway and negatively regulates cytokinin mediated signalling events. Through our induced ectopic expression studies of OsMADS1:ΔGR, we show OsMADS1 directly regulates the expression of OsETTIN2, an auxin response transcription factor, during floret development. Overall, we demonstrate that OsMADS1 modulates hormonal pathways to execute its functions during floret development on the spikelet meristems. Functional studies of OsMGH3; an auxin-responsive indirect target of OsMADS1 To better understand the contribution of auxin signalling during floret development, we have functionally characterized OsMGH3, a down-stream indirect target of OsMADS1, which is a member of the auxin-responsive GH3 family. The members of this family are direct targets of auxin response factors (ARF) class of transcription factors. GH3-proteins inactivate cellular auxin by conjugating them with amino acids and thus regulate auxin homeostasis in Arabidopsis (Staswick et al., 2005). OsMGH3 expression in rice florets overlaps with that of OsMADS1 (Prasad et al, 2005). In this study, we have demonstrated the consequences of OsMGH3 over-expression and knock-down. The over-expression of OsMGH3 during vegetative development causes auxin-deficient phenotypes such as dwarfism and loss of apical dominance. Its over-expression in developing panicles that was obtained by driving its expression from tissue-specific promoters created short panicles with reduced branching. The latter is a phenotype similar to that observed upon over-expression of OsMADS1. In contrast, the down-regulation of endogenous OsMGH3 through RNA-interference produced auxin over-production phenotypes such as ectopic rooting from aerial nodes. Knock-down of OsMGH3 expression in florets affected carpel development and pollen viability both of which affect floret fertility. Taken together, this study provides evidence for the importance of auxin homeostasis and its transcriptional regulation during rice panicle branching and floret organ development. Our analysis of various conserved transcription factors during rice floret development suggest that factors like OsMADS2, OsMADS4 and OsMADS1 are master regulators of gene expression during floret meristem specification and organ development. The target genes regulated by these factors contribute to development of morphologically distinct rice florets.

Gene Expression

Genetic Regulation

Rice Floret Meristem

OsMADS2

OsMADS1

Rice MADS-Box Proteins

Rice PI Like Genes

Gene Transcription

Plant Hormones - Signalling

Auxin

Cytokinin

OsMGH3

Biochemical Genetics

Interpreting Cytokinin Action as Anterograde Signaling and Beyond

Ikeda, Yoshihisa, Zalabák, David, Kubalová, Ivona, Králová, Michaela, Brenner, Wolfram G., Aida, Mitsuhiro

30 March 2023

Among the major phytohormones, the cytokinin exhibits unique features for its ability to positively affect the developmental status of plastids. Even early on in its research, cytokinins were known to promote plastid differentiation and to reduce the loss of chlorophyll in detached leaves. Since the discovery of the components of cytokinin perception and primary signaling, the genes involved in photosynthesis and plastid differentiation have been identified as those directly targeted by type-B response regulators. Furthermore, cytokinins are known to modulate versatile cellular processes such as promoting the division and differentiation of cells and, in concert with auxin, initiating the de novo formation of shoot apical meristem (SAM) in tissue cultures. Yet how cytokinins precisely participate in such diverse cellular phenomena, and how the associated cellular processes are coordinated as a whole, remains unclear. A plausible presumption that would account for the coordinated gene expression is the tight and reciprocal communication between the nucleus and plastid. The fact that cytokinins affect plastid developmental status via gene expression in both the nucleus and plastid is interpreted here to suggest that cytokinin functions as an initiator of anterograde (nucleus-to-plastid) signaling. Based on this viewpoint, we first summarize the physiological relevance of cytokinins to the coordination of plastid differentiation with de novo shoot organogenesis in tissue culture systems. Next, the role of endogenous cytokinins in influencing plastid differentiation within the SAM of intact plants is discussed. Finally, a presumed plastid-derived signal in response to cytokinins for coupled nuclear gene expression is proposed.

info:eu-repo/classification/ddc/570

ddc:570

Genome scale transcriptome analysis and development of reporter systems for studying shoot organogenesis in poplar

Bao, Yanghuan

15 April 2008

Vegetative propagation allows the amplification of selected genotypes for research, breeding, and commercial planting. However, efficient in vitro regeneration and genetic transformation remains a major obstacle to research and commercial application in many plant species. Our aims are to improve knowledge of gene regulatory circuits important to meristem organization, and to identify genes that might be useful for improving the efficiency of in vitro regeneration. In this thesis, we have approached these goals in two ways. First, we analyzed gene expression during poplar (Populus) regeneration using an AffymetrixGeneChip® array representing over 56,000 poplar transcripts. We have produced a catalog of regulated genes that can be used to inform studies of gene function and biotechnology. Second, we developed a GUS reporter system for monitoring meristem initiation using promoters of poplar homologs to the meristem-active regulatory genes WUSCHEL (WUS) and SHOOTMERISTEMLESS (STM). This provides plant materials whose developmental state can be assayed with improved speed and sensitivity. For the microarray study, we hybridized cDNAs derived from tissues of a female hybrid poplar clone (INRA 717-1 B4, Populus tremula x P. alba) at five sequential time points during organogenesis. Samples were taken from stems prior to callus induction, at 3 days and 5 days after callus induction, and at 3 and 8 days after the start of shoot induction. Approximately 15% of the monitored genes were significantly up-or down-regulated based on both Extraction and Analysis of Differentially Expressed Gene Expression (EDGE) and Linear Models for Microarray Data (LIMMA, FDR<0.01). Of these, over 3,000 genes had a 5-fold or greater change in expression. We found a very strong and rapid change in gene expression at the first time point after callus induction, prior to detectable morphological changes. Subsequent changes in gene expression at later regeneration stages were more than an order of magnitude smaller. A total of 588 transcription factors that were distributed in 45 gene families were differentially regulated. Genes that showed strong differential expression encoded proteins active in auxin and cytokinin signaling, cell division, and plastid development. When compared with data on in vitro callogenesis from root explants in Arabidopsis, 25% (1,260) of up-regulated and 22% (748) of down- regulated genes were in common with the genes that we found regulated in poplar during callus induction. When ~3kb of the 5' flanking regions of close homologs were used to drive expression of the GUSPlus gene, 50 to 60% of the transgenic events showed expression in apical and axillary meristems. However, expression was also common in other organs, including in leaf veins (40% and 46% of WUS and STM transgenic events, respectively) and hydathodes (56% of WUS transgenic events). Histochemical GUS staining of explants during callogenesis and shoot regeneration using in vitro stems as explants showed that expression was detectable prior to visible shoot development, starting 3 to 15 days after explants were placed onto callus inducing medium. Based on microarray gene expression data, a paralog of poplar WUS was detectably up-regulated during shoot initiation, but the other paralog was not. Surprisingly, both paralogs of poplar STM were down-regulated 3- to 6-fold during early callus initiation, a possible consequence of its stronger expression in the secondary meristem (cambium) than in shoot tissues. We identified 15 to 35 copies of cytokinin response regulator binding motifs (ARR1AT) and one copy of the auxin response element (AuxRE) in both promoters. Several of the WUS and STM transgenic events produced should be useful for monitoring the timing and location of meristem development during natural and in vitro shoot regeneration. / Graduation date: 2008

Populus

in vitro shoot organogenesis

transcriptome

auxin

cytokinin

transformation

regeneration

WUS

STM

meristem

secondary meristem

cambium

promoter

stem cells

Poplar -- Genetics

Poplar -- Regeneration

Poplar -- Growth -- Regulation

Plant genetic regulation

Plant hormones

Meristems

Caractérisation de la voie TCTP (TRANSLATIONALLY CONTROLLED TUMOR PROTEIN) chez Arabidopsis thaliana : identification des régulateurs de son accumulation et importance de la voie au cours du développement embryonnaire / Characterization of the TCTP (TRANSLATIONALLY CONTROLLED TUMOR PROTEIN) pathway in Arabidopsis thaliana : identification of TCTP accumulation regulators and importance of the pathway during embryo development

Savarin, Julie

02 March 2018

TCTP (Translationally Controlled Tumor Protein) est une protéine très conservée chez l'ensemble des eucaryotes. C’est une protéine vitale impliquée dans divers processus essentiels, et pour de nombreux organismes son absence conduit à la létalité dès les stades embryonnaires.Chez les animaux comme chez les végétaux, TCTP joue un rôle primordial dans la croissance et le développement des individus. En plus de son implication dans l’apoptose et la réparation de l’ADN, TCTP favorise la prolifération cellulaire, et se trouve donc être un élément important de la tumorigenèse. Chez les végétaux, la forte conservation de TCTP a permis la préservation de la plupart des fonctions décrites chez les animaux, mais les facteurs qui interviennent en amont ne sont pas encore connus.Par la mise en place, la conduite et la finalisation de deux cribles génétiques utilisant la plante modèle Arabidopsis thaliana, ce travail de thèse a cherché à identifier des facteurs situés en amont de TCTP. En parallèle, une seconde étude fut menée afin de mesurer l'impact de l'absence de TCTP sur les voies de l’auxine et des cytokinines au cours du développement embryonnaire, permettant de mieux comprendre l’origine de l’embryolétalité du mutant tctp. / TCTP (Translationally Controlled Tumor Protein) is strongly conserved among eukaryotes. It is a vital protein implicated in various major processes, and its absence leads to early embryolethality in many organisms. In plants as in animals, TCTP is a key factor of growth and development. Implicated in apoptosis and DNA repair, TCTP is also an enhancer of cell proliferation, and is a key element of tumorigenesis. Major functions of TCTP are conserved between plants and animals, but upstream factors are not known yet. Using a genetic screen on the model plant Arabidopsis thaliana, the principal goal of this thesis was to discover regulators of TCTP.In parallel, the impact of TCTP knockout on auxin and cytokinin pathways during embryo development was investigated.

Arabidopsis thaliana

Génétique

Méthanesulfonate d'éthyle

Cycle cellulaire

Biologie Végétale

Cytokinine

Plantes -- Développement

Arabidopsis thaliana

Genetic

Ethyl Methanesulfonate (EMS)

Cell cycle

Plant Biology

Cytokinin

Plants — Development

Etude du rôle de AHP6 dans le contrôle de la phyllotaxie chez la plante modèle Arabidopsis thaliana : robustesse et coordination spatio-temporelle au cours du développement de structures auto-organisées / Study of the role of AHP6 in the control of phyllotaxis in Arabidopsis thaliana : robustness and spatio-temporal coordination in the development of self-organized organisms

Besnard, Fabrice

21 October 2011

En se développant, les plantes produisent des organes le long des tiges suivant des organisations stéréotypées, appelées phyllotaxies. Ces structures se forment dans les méristèmes, qui abritent une niche de cellules souches : les organes y sont produits successivement et leur positionnement dépendrait d'interactions dynamiques avec les organes pré-existants. Ces interactions seraient notamment dues à des champs inhibiteurs générés par le transport polaire de l'hormone végétale auxine. Afin de rechercher si d'autres facteurs que l'auxine contrôlent la phyllotaxie chez Arabidopsis thaliana, nous nous sommes intéressés au rôle possible des cytokinines, une autre hormone végétale. Nous avons développé des nouvelles méthodes statistiques pour analyser la structure de la phyllotaxie. Cette approche nous a permis d'identifier des anomalies de phyllotaxie chez des plantes mutantes pour le gène AHP6 (ARABIDOPSIS HISTIDINE PHOSPHOTRANSFER protein 6), un inhibiteur de la signalisation des cytokinines. Notre analyse suggérait des possibles perturbations du plastochrone, la période de temps séparant l'initiation de deux organes, ce que nous avons alors confirmé par imagerie confocale en temps réel. Nos données montrent que AHP6 contrôle la régularité du plastochrone, et suggèrent que les perturbations de phyllotaxies sont dues à l'initiation simultanée de deux à trois organes dans le méristème. De plus, AHP6 est exprimé dans les organes et sa protéine établit des champs qui inhibent la signalisation des cytokinines au delà des organes. Pour mieux comprendre les rôles possibles de ces champs, nous avons généré un modèle numérique théorique de la phyllotaxie. Notre étude suggère que le plastochrone pourrait être déstabilisé par du bruit affectant le seuil d'activation nécessaire aux cellules méristématiques pour se différencier en organe. Des champs inhibiteurs pourraient filtrer les effets de ce bruit en influant sur la cinétique d'émergence des organes. Les propriétés observées des champs de AHP6 sont en accord avec ce modèle et nos données expérimentales suggèrent en effet que AHP6 et les cytokinines peuvent moduler la signalisation auxine lors de l'émergence des organes. Nous proposons comme modèle que le transport et la signalisation de l'auxine positionnent de manière robuste les organes mais génèrent un plastochrone irrégulier en présence de bruit. Des champs inhibiteurs de cytokinines stabiliseraient le plastochrone, assurant un couplage plus robuste entre le temps et l'espace lors de l'établissement de la phyllotaxie. / During development, plant aerial organs are produced along the stems following stereotyped patterns. This so-called phyllotaxis is initiated at the shoot meristem, which contains the stem cell niche: organs are produced iteratively and their precise position is thought to depend on dynamic interactions with preexisting organs. These interactions would notably result from inhibitory fields generated by the polar transport of the plant hormone auxin. To investigate whether other factors than auxin regulate phyllotaxis, we studied the potential role of cytokinin signaling. We developed a new pipeline of methods based on statistics to analyze phyllotactic patterns. This approach allowed us to identify phyllotactic perturbations in mutants of the AHP6 (ARABIDOPSIS HISTIDINE PHOSPHOTRANSFER protein 6), an inhibitor of cytokinin signaling that suggested perturbations in the plastochron, the time between two organ initiations. This was further confirmed using confocal live-imaging. We demonstrated that AHP6 controls the regularity of the plastochron, and our results suggest that the defective phyllotaxis in ahp6 is caused by concomitant initiations of two or three organs in the meristem. Interestingly, AHP6 is expressed in organs and the protein can move beyond these domains, generating cytokinin signaling inhibitory fields. To explore further the putative role of these secondary fields, we generated a mathematical model of phyllotaxis. This suggested that plastochron instabilities could be caused by noise affecting the threshold at which meristematic cells are recruited into organs. Inhibitory fields generated by AHP6 could filter out the effect of noise by modifying the kinetics of early organ emergence. Consistently, the properties of AHP6 fields fit the model predictions and our experimental data show that AHP6 and cytokinin modulate auxin signaling during organ emergence. We thus propose a model in which auxin transport and signaling robustly control organ positioning but generates plastochron instablities in noisy backgrounds. In this scenario cytokinin inhibitory fields would stabilize the rhythmicity of organ initiation, ensuring a robust coupling of space and time during pattern formation.

Phyllotaxie

Méristème apical caulinaire

Interactions auxine-cytokinine

Arabidopsis

Champs inhibiteur

Bruit et robustesse

Motifs de développement

Modèle de systèmes dynamiques

Analyses de motifs

Phyllotaxis

Shoot apical meristem

Auxin-cytokinin crosstalk

Arabidopsis

Inhibitory fields

Noise and robustness

Developmental pattern

Dynamical system model

Pattern analysis

Transport a metabolismus radioaktivně značených cytokininů v rostlinných buňkách a pletivech / Transport and Metabolism of Radio-Labelled Cytokinins in Plant Cells and Tissues

Nedvěd, Daniel

January 2020

Cytokinins are a large group of phytohormones. Since their discovery in the 1950s, they have shown to play a pivotal role in plant physiology. Most studies so far focused on cytokinin action mechanisms and their metabolic regulation. Identification of AtABCG14 and AtPUP14 as cytokinin-specific membrane carriers brought researchers' attention to cytokinin membrane transport, too. In this thesis, we performed experiments with radio-labelled cytokinin tracers. We show that trans-zeatin and isopentenyladenine, two major biologically active cytokinins, are readily transported across the plasma membrane in tobacco BY-2 cell suspension. Making use of mathematical modelling, we show that BY-2 cells possess a membrane transport system with an affinity toward cytokinins. Next, we show that atabcg14 and atpup14 mutations affect cytokinin metabolism in Arabidopsis thaliana plants. Keywords: cytokinin, Arabidopsis thaliana, tobacco BY-2 cell lines, membrane transport, purine permease, ATP-binding cassette, radio-labelling

Manejo pós-colheita de Alpinia purpurata (Vieill) K. Schum (Zingiberaceae)

Silva, Antonio Tarciso Ciríaco da

22 March 2006

The growth of ornamental plant market in Brazil is remarkable nowadays with strong participation of Northeast region, particularly in Alagoas State on the commercialization of tropical flowers. Taking into account this economic aspect, it is of great importance for the productive chain of ornamental species the study of aspects of post harvest activities. Alpinia purpurata (Viell) K. Schum (Zingiberaceae) which occupies the second place in economic importance amongst tropical flowers. It is the main flower for growing and harvesting. The main objective of this research programme is to study the different aspects of Alpinia post-harvesting: (1) time of harvesting and cut of the basis of the stems, and (2) the use of solutions of pulsing ; and/or maintenance of the floral stem by using: (2.1.) biocide compounds and pH of the solution; (2.2) carbohydrates and carbohydrates plus biocides; (2.3) anti-ethylene compounds and antiethylene compounds plus carbohydrates; (2.4) elements as calcium and silicon; and (2.5) senescence retarding growth regulators. It was evaluated the influence of these factors in the water relations, quality and longevity of the stems. Six experiments were carried out in the laboratory (CECA) of the Federal University of Alagoas. In the first experiment, the stems were harvested in three different times and they were cut periodically on their basis. In the second experiment different biocide substances were tested (8- hydroxyquinoline sulphate, aluminum sulphate, salicilic acid and sodium hipocloride) associated to pH variation of the maintenance solution. In the third experiment the stems received sucrose solutions pulsing from 2 to 20% for 12, 24 and 48 hours, following by maintenance in distilled water or in solution of 8- hidroxikinolin (HQS). The fourth experiment comprised three times of exposition (30, 60 and 120 min) with STS 1mM following by the presence or absence of pulsing in sucrose 20% for 12 hours. In the fifth experiment it was evaluated the effect of the addition of Ca (calcium sulphate 50 and 100mM), Si (sodium silicate 1,25 and 2,50 mM) and Ca+Si in maintenance solution. In the sixth experiment the stems were submitted to gibberellins, solutions (GA3), 10, 30 and 60 μm and cytokinin (benzyladenine 6-BA), 10, 20 and 100μm in 24 hours pulsing under continuous light. In all experiments the fresh biomass and the quality (scale of values) of the stems were determined daily or every two days until the end of the experiment. The amount of water was also determined for the floral bracts and dry biomass. The experiments were analised by completely randomized design and the data submitted to the variance analysis, test of averages and , when necessary, to the regression analysis. It was observed that the stems harvested at the end of the afternoon had shown greater commercial value; however, the regular cuts of the basis of the stems reduced their longevity. The use of HQS provided greater durability and humidity of the stems. On the other hand the other biocides did not improve the quality when compared to the control. The reduction of the pH by using citric acid did not interfere with the studied parameters. The use of sucrose in pulsing was only effective when the stems had been kept in distilled water. In this case the concentration sucrose of 20% for 12 hours showed better results. Silver thiosulphate when in pulsing for 30 minutes produced an increase of water contents and for 60 minutes or plus, or when addition of sucrose, caused dehydration of the stems. The only use of calcium sulphate or in association with sodium silicate in maintenance solution caused high improvement of the quality of the stems in comparison to the control and sodium silicate treatment. The use of cytokinin and gibberellins even considering it improved the water contents of the stems did not affect the commercial durability of them. / É notável o crescimento do mercado de plantas ornamentais no Brasil. Com participação efetiva da região Nordeste, destacando-se as exportações de flores tropicais, onde o Estado de Alagoas vem se firmando, com Alpinia purpurata (Viell) K. Schum (Zingiberaceae) como a principal flor de corte, e que ocupa o segundo lugar em importância econômica dentre as flores tropicais. Levando-se em conta esse aspecto econômico, verifica-se ser de grande importância para a cadeia produtiva desses cultivos, o estudo de aspectos relativos à da pós-colheita. Assim sendo, a presente pesquisa, objetivou estudar diferentes aspectos do manejo pós-colheita dessas flores, testando: (1) hora de colheita e corte da base das hastes, e (2) o uso de soluções de pulsing ; e/ou manutenção das hastes florais - neste caso ainda associado (2.1) a substâncias biocidas com o pH na solução sob controle; (2.2) a carboidratos e carboidratos mais biocidas; (2.3) a substâncias anti-etileno e substâncias anti-etileno mais carboidratos; (2.4) a elementos como cálcio e silício; e (2.5) a fitorreguladores retardantes da senescência. Avaliou-se a influência destes fatores nas relações hídricas, qualidade e longevidade das hastes cortadas, através de seis experimentos em laboratório no Centro de Ciências Agrárias da Universidade Federal de Alagoas (CECA/UFAL). No primeiro experimento, as hastes foram colhidas em três diferentes horários, recebendo durante o período pós-colheita cortes periódicos na base da haste. No segundo experimento, foram testadas substâncias biocidas (Sulfato de 8- hidroxiquinolina, Sulfato de alumínio, Ácido salicílico, Hipoclorito de sódio) associadas à redução ou não do pH. No terceiro experimento as hastes receberam tratamento de pulsing com soluções de sacarose entre 2 e 20%, por períodos de 12, 24 e 48 h, seguidas de manutenção em água destilada ou em solução de 8-hidroxiquinolina (HQS) comparando-se com duas testemunhas (água destilada ou solução de HQS). No quarto experimento, foram testados três tempos de exposição (30, 60 e 120 minutos) a STS 1mM, seguido ou não de pulsing em sacarose a 20%, por 12 horas. No quinto experimento, foram verificados os efeitos da adição de Ca (sulfato de cálcio a 50 e 100mM), Si ( silicato de sódio a 1,25 e 2,50 mM) e Ca+Si em solução de manutenção. No sexto experimento, as hastes foram submetidas a soluções de SILVA, A.T.C. 2006 Manejo pós-colheita de alpinia purpurata (Vieill) K. Schum (zingiberaceae)... xv giberelina (GA3), a 10, 30 e 60 μM e citocinina (benziladenina 6-BA), a 10, 20 e 100 μM em pulsing por 24 horas, sob luz contínua. Em todos os experimentos, a massa fresca e a qualidade (com base em notas) das hastes foram determinadas diariamente, ou a cada 2 dias; no final de cada experimento foram também determinados o conteúdo relativo de água das brácteas florais e a massa seca das hastes. O delineamento utilizado foi o inteiramente casualizado sendo os dados submetidos à análise de variância, teste de médias e, quando necessário, à análise de regressão. As hastes cortadas ao final da tarde tiveram maior durabilidade comercial, porém o corte periódico da base das hastes reduziu sua longevidade. O uso de HQS proporcionou maior durabilidade e hidratação das hastes, sendo que os demais biocidas testados não melhoraram a qualidade. A redução do pH, pelo uso do ácido cítrico, não influenciou nas variáveis estudadas. O uso de sacarose em pulsing só foi efetivo quando as hastes foram mantidas em água destilada, sendo melhor o resultado para a concentração de 20% por 12 horas. O tiossulfato de prata em pulsing por 30 minutos, promoveu um aumento de hidratação, mas desidratou as hastes a 60 minutos ou mais ou quando adicionado à sacarose. O uso de sulfato de cálcio em solução de manutenção e quando associado ao silicato de sódio promoveu elevada melhoria de qualidade das hastes. O uso de citocininas e giberelinas embora tenha melhorado as relações hídricas das hastes não afetou a durabilidade comercial das mesmas.

Harvesting time

Recutting stems

8-hydroxyquinoline sulphate (HQS)

Sucrose

Silver thiosulphate (STS)

Calcium sulphate

Sodium silicate

Gibberellins (GA3)

Cytokinin (benzyladenine - 6-BA)

Horário de colheita

Recorte das hastes

Sulfato de Hidroxiquinolina (8-HQS)

Sacarose

Tiosulfato de prata (STS)

Sulfato de cálcio

Silicato de sódio

Giberelina (GA3)

Benziladenina (6-BA)

CNPQ::CIENCIAS AGRARIAS::AGRONOMIA

Identification de facteurs de transcription régulateurs de la voie de biosynthèse des alcaloïdes indoliques monoterpéniques chez Catharanthus roseus / Identification of transcription factors regulating the biosynthesis pathway of monoterpene indole alkaloids in catharanthus roseus

Ginis, Olivia

08 June 2012

Catharanthus roseus est une plante tropicale qui produit spécifiquement des alcaloïdes indoliques monoterpéniques (AIM) d’intérêt thérapeutique. Chez C. roseus, la branche terpénique incluant la voie du méthylérythritol phosphate (MEP) est considérée comme limitante et présente une régulation transcriptionnelle coordonnée en réponse aux hormones inductrices de l’accumulation alcaloïdique. Lors de ce travail, suite à des analyses bioinformatiques et à la caractérisation de promoteurs de gènes de la voie MEP, nous avons identifié de nouvelles familles de facteurs de transcription impliquées dans la régulation de la biosynthèse des AIM. Des membres de la famille des ZCT, des WRKY et des RR type B interagissent avec le promoteur du gène hds de la voie MEP et régulent son activité. Ces travaux ont permis d’approfondir les connaissances sur les réseaux transcriptionnels régulateurs de la biosynthèse des AIM. L’utilisation de ces nouveaux facteurs de transcription activateurs peut désormais être envisagée dans le cadre d’expériences d’ingénierie métabolique afin d’augmenter l’accumulation d’alcaloïdes d’intérêt pharmaceutique chez C. roseus. / Catharanthus roseus is a tropical plant producing specifically monoterpene indole alkaloids (MIA) of high interest due to their therapeutical values. In C. roseus cells, the terpenoid branch including the methyl erythritol phosphate pathway (MEP) provides the MIA terpenoid moiety and is regarded as limited for MIA biosynthesis. This branch presents a coordinated transcriptional regulation in response to hormonal signals leading to MIA production. In this context, bioinformatic analysises and functional characterization of MEP pathway gene promoters allowed the identification of new transcription factor families involved in the MIA pathway regulation. Members of ZCT proteins, WRKY and type B RR families specifically interact with the hds promoter from the MEP pathway and regulate its activity. This work permits to gain into insight the transcriptional network controlling the MIA biosynthesis. It is possible now to consider using transcription factor that act as activators and target genes from the terpenoid branch to increase the accumulation of alkaloids of pharmaceutical interest in C. roseus by metabolic engineering approaches.

Catharanthus roseus

Cultures cellulaires

Alcaloïdes indoliques monoterpéniques

Terpènes

MEP

Promoteur

Facteur de transcription

Phytohormones

Signalisation cytokinine

Biolistique

Criblage par simple hybride de levure

Ingénierie métabolique

Méthylérytritol Phosphate

Catharanthus roseus

Cell cultures

Monoterpene indole alkaloids

Terpanoid

MEP

Promoter

Transcription factor

Plant hormones

Cytokinin signaling

Boilistic

Yeast one-hybrid screening

Metabolic engineering

Origin & Evolution of the C3HDZ-ACL5-SACL Regulatory Module in Land Plants

Solé Gil, Anna

07 September 2023

[ES] El correcto desarrollo de tejidos vasculares depende del ajuste preciso entre la proliferación de células vasculares y la diferenciación celular. En Arabidopsis thaliana, la proliferación de células vasculares en el cambium es potenciada por la citoquinina, la síntesi de la cual está promovida por la actividad dependiente de auxina de un heterodímero de factores de transcripción (TF) formado por LONESOME HIGHWAY (LHW) y por TARGET OF MONOPTEROS 5 (TMO5). Como mecanismo de seguridad, las auxinas también activan un módulo inhibidor que implica la inducción precisa de la Termospermina (Tspm) sintasa ACAULIS5 (ACL5) en células vasculares proliferantes por acción conjunta de las auxinas y del TF Class III HD-ZIP (C3HDZ) AtHB8. Entonces, la Tspm permite la traducción de las proteínas SACL de forma celular autónoma, que perjudican la actividad de LHW. Sin embargo, la observación de que estos elementos están presentes en los genomas de todas las plantas terrestres - y no sólo de las plantas vasculares - plantea dos preguntas desde una perspectiva evolutiva: (i) ¿cuál es la función de estos genes en las plantas terrestres no vasculares? y (ii) ¿cuándo se creó el módulo regulador concreto? En esta Tesis, mediante la combinación de análisis filogenéticos, celulares y moleculares con la hepática Marchantia polymorpha, proponemos que la auxina y C3HDZ son reguladores ancestrales de la expresión de ACL5, y que esta conexión se mantiene en las traqueófitas y las briófitas existentes. Por el contrario, la traducción dependiente de Tspm de SACL parece ser específica de las traqueófitas, basado en la aparición de un uORF conservado en la secuencia 5' líder de los tránscritos de SACL y en evidencia experimental basada en ensayos transitorios para la traducción de SACL. De acuerdo con estas observaciones, las funciones de MpACL5 y MpSACL son diferentes en M. polymorpha. MpACL5 se expresa en "notches" apicales y modula la bifurcación de los meristemos. Por otro lado, la expresión de MpSACL está mayoritariamente excluida de los "notches" apicales y su actividad afecta negativamente la producción de gemas y rizoides mediante la interacción con MpRSL1. Finalmente, la hibridación de ARN in situ de ortólogos de C3HDZ, ACL5 y SACL en la gimnosperma Ginkgo biloba, el helecho Ceratopteris richardii y la licófita Selaginella kraussiana indican que la expresión de los tres genes se solapa en los tejidos vasculares. Nuestros resultados sugieren que la función de C3HDZ, ACL5 y SACL ha seguido trayectorias evolutivas divergentes en briófitas y traqueófitas, para controlar, finalmente, diferentes funciones específicas dentro de cada linaje. Sólo en las traqueófitas se formó el módulo regulador y se asoció con la restricción de la proliferación de células vasculares. / [CA] El correcte desenvolupament dels teixits vasculars depèn del precís ajust entre la proliferació de cèl·lules vasculars i la diferenciació cel·lular. En Arabidopsis thaliana, la proliferació de cèl·lules vasculars al càmbium és potenciada per la citoquinina, la síntesi de la qual està promoguda per l'activitat dependent d'auxina d'un heterodímer de factors de transcripció (TF) format per LONESOME HIGHWAY (LHW) i TARGET OF MONOPTEROS 5 (TMO5). Com a mecanisme de seguretat, l'auxina també activa un mòdul inhibidor que implica la inducció precisa de la Termospermina (Tspm) sintasa ACAULIS5 (ACL5) en cèl·lules vasculars proliferants per l'acció conjunta de l'auxina i del TF Class III HD-ZIP (C3HDZ) AtHB8. Llavors, la Tspm permet la traducció de les proteïnes SACL de forma autònoma cel·lular, que perjudiquen l'activitat de LHW. Tanmateix, l'observació de que aquests elements estan presents en els genomes de totes les plantes terrestres - i no només de les plantes vasculars - planteja dues preguntes des d'una perspectiva evolutiva: (i) quina és la funció d'aquests gens en les plantes terrestres no vasculars? i (ii) quan es va crear el mòdul regulador complet? En aquesta Tesi, mitjançant la combinació d'anàlisis filogenètics, cel·lulars i moleculars amb la hepàtica Marchantia polymorpha, proposem que l'auxina i C3HDZ són reguladors ancestrals de l'expressió d'ACL5, i que aquesta connexió es mantén en els traqueòfits i briòfits existents. Per contra, la traducció depenent de Tspm de SACL sembla ser específica dels traqueòfits, basat en l'aparició d'un uORF conservat a la seqüència 5' líder dels trànscrits de SACL i en evidència experimental basada en assajos transitoris per a la traducció de SACL. D'acord amb aquestes observacions, les funcions de MpACL5 i MpSACL són diferents a M. polymorpha. MpACL5 s'expressa en "notch" apicals i modula la bifurcació dels meristems. D'altra banda, l'expressió de MpSACL està majoritàriament exclosa dels "notch" apicals i la seva activitat afecta negativament la producció de gemmes i rizoids mitjançant la interacció amb MpRSL1. Finalment, la hibridació d'ARN in situ d'ortòlegs de C3HDZ, ACL5 i SACL a la gimnosperma Ginkgo biloba, la falguera Ceratopteris richardii i el licòfit Selaginella kraussiana indica que l'expressió dels tres gens es solapa als teixits vasculars. Els nostres resultats suggereixen que la funció de C3HDZ, ACL5 i SACL va seguir trajectòries evolutives divergents en briòfits i traqueòfits, per controlar, finalment, diferents funcions específiques dins de cada llinatge. Només en els traqueòfits es va formar el mòdul regulador i es va associar amb la restricció de la proliferació de cèl·lules vasculars. / [EN] The correct development of vascular tissues depends on the precise adjustment between vascular cell proliferation and cell differentiation. In Arabidopsis thaliana, vascular cell proliferation in the cambium is enhanced by cytokinin, whose synthesis is promoted by the auxin-dependent activity of a transcription factor (TF) heterodimer formed by LONESOME HIGHWAY (LHW) and TARGET OF MONOPTEROS 5 (TMO5). As a safety mechanism, auxin also deploys a negative feedforward regulatory module which involves the precise induction of the Thermospermine (Tspm) synthase ACAULIS5 (ACL5) in proliferating vascular cells by the joint action of auxin and the class-III HD-ZIP (C3HDZ) AtHB8 TF. Tspm then allows the cell-autonomous translation of the SACL proteins, which impair the activity of LHW. However, the observation that these elements are present in the genomes of all land plants -and not only vascular plants- poses two questions from an evolutionary perspective: (i) what is the function of these genes in non-vascular land plants? and (ii) when was the full regulatory module assembled? In this Thesis, through the combination of phylogenetic, cellular, and molecular genetic analyses with the liverwort Marchantia polymorpha, we propose that auxin and C3HDZ are ancestral regulators of ACL5 expression, and that this connection is maintained in extant tracheophytes and bryophytes. On the contrary, thermospermine-dependent translation of SACL seems to be specific of tracheophytes, based on the appearance of a conserved uORF in the 5' leader sequence of SACL transcripts and on experimental evidence using transient assays for SACL translation. In agreement with these observations, the functions of MpACL5 and MpSACL are different in M. polymorpha. MpACL5 is expressed in apical notches and modulates meristem bifurcation. On the other hand, MpSACL expression is mostly excluded from apical notches and its activity negatively affects gemmae and rhizoid production through the interaction with MpRSL1. Finally, in situ RNA hibridization of C3HDZ, ACL5 and SACL orthologs in the gymnosperm Ginkgo biloba, the fern Ceratopteris richardi and the lycophyte Selaginella kraussiana indicates that the expression of the three genes overlaps in vascular tissues. Our results suggest that the function of C3HDZ, ACL5 and SACL followed divergent evolutionary trajectories in bryophytes and tracheophytes, to ultimately control different lineage-specific functions. Only in tracheophytes was the regulatory module assembled and associated with the restriction of vascular cell proliferation. / Solé Gil, A. (2023). Origin & Evolution of the C3HDZ-ACL5-SACL Regulatory Module in Land Plants [Tesis doctoral]. Universitat Politècnica de València. https://doi.org/10.4995/Thesis/10251/196681

ACAULIS5 (ACL5)

Plantas terrestres

Plantas vasculares

Briofitas

Termospermina

Desarrollo vascular

Xilema

Biología molecular

Biotecnología

Red de regulación génica

Auxina

Citoquinina

Poliaminas

Evolution

Land Plants

Vascular Plants

Bryophytes

C3HDZ

SACL

Thermospermine

Marchantia polymorpha

Arabidopsis thaliana

Ginkgo biloba

Ceratopteris richardii

Selaginella kraussiana

Vascular development

Xylem

Molecular Biology

Biotechnology

Gene regulatory network

Auxin

Cytokinin

Polyamines

upstream Open Reading Frame (uORF)

FISIOLOGIA VEGETAL