Etude génétique et moléculaire de deux gènes de Medicago truncatula, DMI3 et RPG, contrôlant l'établissement de symbioses racinaires

Godfroy, Olivier Rosenberg, Charles Debelle, Frédéric

January 2008

Reproduction de : Thèse de doctorat : Biosciences végétales : Toulouse 3 : 2008. / Titre provenant de l'é215-232.

Quantification of the belowground inputs of organic carbon by the annual pasture legume barrel medic (Medicago truncatula Gaertn.) / by Michael Cameron Crawford.

Crawford, Michael Cameron

January 1997

Bibliography: leaves 164-193. / x, 193 leaves : ill. ; 30 cm. / Title page, contents and abstract only. The complete thesis in print form is available from the University Library. / This study aims to quantify the belowground input of organic carbon by barrel medic using techniques that account for root death and decomposition as well as root secretion and exudation. It also investigates the effect of defoliation on carbon allocation within the plant so as to determine the potential for optimising carbon input to the soil through grazing management. / Thesis (Ph.D.)--University of Adelaide, Dept. of Soil Science, 1997

Medicago South Australia.

Soils South Australia Carbon content.

Defoliation.

Humus.

Soil management.

Why are the symbioses between some genotypes of Sinorhizobium and Medicago suboptimal for N2 fixation?

J.Terpolilli@murdoch.edu.au, Jason Terpolilli

January 2009

The conversion of atmospheric dinitrogen (N2) into plant available nitrogen (N), by legumes and their prokaryotic microsymbionts, is an integral component of sustainable farming. A key constraint to increasing the amount of N2 fixed in agricultural systems is the prevalence of symbioses which fix little or no N. The biotic factors leading to this suboptimal N2 fixation have not been extensively analysed. Using the widely studied and cultivated perennial legume Medicago sativa and the model indeterminate annual legume Medicago truncatula with the sequenced bacterial microsymbiont Sinorhizobium meliloti 1021 (Sm1021) as a basis, the work presented in this thesis examined the effectiveness of N2 fixation in these associations and in other comparable systems and investigated factors which lead to the establishment of suboptimally effective symbioses. The ability of Sm1021, S. medicae WSM419 and the uncharacterised Sinorhizobium sp. WSM1022 to fix N with M. truncatula A17, M. sativa cv. Sceptre and a range of other Medicago spp. was evaluated in N-limited conditions. As measured by plant shoot dry weights and N-content, Sm1021 was partially effective with M. truncatula A17 whereas WSM1022 and WSM419 were both effective with this host in comparison to nitrogen-fed (N-fed) control plants. In contrast, Sm1021 and WSM1022 were effective with M. sativa while WSM419 was only partially effective. Nodules induced by Sm1021 on M. truncatula A17 were more numerous, paler, smaller in size and more widely distributed over the entire root system than in the two effective symbioses with this host. On the contrary, nodule number, size and distribution did not differ between these three strains on M. sativa. WSM1022 was effective on M. littoralis, M. tornata and two other cultivars of M. truncatula (Jemalong and Caliph) but Sm1021 was only partially effective on these hosts. These data indicate that the model indeterminate legume symbiosis between M. truncatula and Sm1021 is not optimally matched for N2 fixation and that Sm1021 possesses broader symbiotic deficiencies. In addition, the interaction of WSM1022 with M. polymorpha (small white nodules but does not fix N), M. murex (does not nodulate), M. arabica (partially effective N2 fixation) and M. sphaeorcarpus (partially effective N2 fixation), and the sequence of the 16S rDNA, are all consistent with this isolate belonging to the species S. meliloti. The colony morphology of TY, half-LA and YMA agar plate cultures of Sm1021, WSM419 and WSM1022 suggested differences in EPS profiles between these strains. Sm1021 is very dry, compared to the mucoid WSM419 and extremely mucoid WSM1022. Sm1021 is known to carry an insertion in expR rendering the gene non-functional and resulting in the dry colony phenotype. WSM419 has an intact copy of expR, while the expR status of WSM1022 is not known. Rm8530, a spontaneous mucoid derivative of Sm1021 with an intact expR, was significantly less effective with M. truncatula than Sm1021, but there was no difference in effectiveness between these strains on M. sativa. The effectiveness of Sm1021, when complemented with a plasmid-borne copy of expR from Rm8530, was significantly reduced on M. truncatula but not M. sativa, implicating a functional expR as being the cause of reduced N2 fixation observed with Rm8530 on M. truncatula. ExpR could reduce the effectiveness of Rm8530 by acting as a negative regulator of genes essential for symbiosis with M. truncatula, or by altering the quantity or structure of succinoglycan and/or galactoglucan produced. These data support the emerging view of ExpR being a central regulator of numerous cellular processes. The timing of nodulation between Sm1021 and WSM419 on M. truncatula and M. sativa was investigated. Compared to the other symbioses analysed, the appearance of nodule initials and nodules was delayed when M. truncatula was inoculated with Sm1021 by 3 and 4 days, respectively. To explore whether events during early symbiotic signalling exchange could account for these observed delays, leading to the establishment of a suboptimal N2-fixing symbiosis, a novel system was developed to compare the response of the Sm1021 transcriptome to roots and root exudates of M. truncatula A17 and M. sativa cv. Sceptre. This system consisted of a sealed 1 L polycarbonate chamber containing a stainless steel tripod with a wire mesh platform on which surface-sterilised seeds could be placed and allowed to germinate through the mesh, into a hydroponic medium below. After germination, Sm1021 cells were inoculated into the hydroponic solution, exposed to the roots and root exudates for 16 h, harvested and their RNA extracted. Comparison of Sm1021 mRNA from systems exposed to M. truncatula or M. sativa revealed marked differences in gene expression between the two. Compared to the no plant control, when M. sativa was the host plant, 23 up-regulated and 40 down-regulated Sm1021 genes were detected, while 28 up-regulated and 45 down-regulated genes were detected with M. truncatula as the host. Of these, 12 were up-regulated and 28 were down-regulated independent of whether M. truncatula or M. sativa was the host. Genes expressed differently when exposed to either M. truncatula or M. sativa included nex18, exoK, rpoE1 and a number of other genes coding for either hypothetical proteins or proteins with putative functions including electron transporters and ABC transporters. Characterisation of these differentially expressed genes along with a better understanding of the composition of M. truncatula root exudates would yield a clearer insight into the contribution of early signal exchange to N2 fixation. Comparison of the regulation of nodule number between Sm1021 and WSM419 on M. truncatula and M. sativa revealed nodule initials at 42 days post-inoculation (dpi) on M. truncatula inoculated with Sm1021. In contrast, no new nodule initials were present 21 dpi on any of the other interactions examined. Moreover, analysis of nodule sections revealed that the number of infected cells in M. truncatula-Sm1021 nodules was less than for comparable symbioses. These data suggest that nodule number is not tightly controlled in the M. truncatula-Sm1021 association, probably due to N2 fixation being insufficient to trigger the down regulation of nodulation. Quantification of N2 fixation activity in this and other more effective symbioses is required. The poor effectiveness of the M. truncatula-Sm1021 symbiosis makes these organisms unsuitable as the model indeterminate interaction and the implications for legume research are discussed. The recently sequenced WSM419 strain, revealed here to fix N2 more effectively with M. truncatula than Sm1021, may be a better model microsymbiont, although WSM419 is only partially effective for N2 fixation with M. sativa. The sequencing of S. meliloti WSM1022, a highly effective strain with both M. truncatula and M. sativa, would provide a valuable resource in indentifying factors which preclude the establishment of effective symbioses.

Root Nodule Bacteria

Effectiveness

Model Legume

Medicago truncatula

Sinorhizobium meliloti

Sinorhizobium medicae

Quantification of the belowground inputs of organic carbon by the annual pasture legume barrel medic (Medicago truncatula Gaertn.) / by Michael Cameron Crawford.

Crawford, Michael Cameron

January 1997

Bibliography: leaves 164-193. / x, 193 leaves : ill. ; 30 cm. / Title page, contents and abstract only. The complete thesis in print form is available from the University Library. / This study aims to quantify the belowground input of organic carbon by barrel medic using techniques that account for root death and decomposition as well as root secretion and exudation. It also investigates the effect of defoliation on carbon allocation within the plant so as to determine the potential for optimising carbon input to the soil through grazing management. / Thesis (Ph.D.)--University of Adelaide, Dept. of Soil Science, 1997

Medicago South Australia.

Soils South Australia Carbon content.

Defoliation.

Humus.

Soil management.

Biochemical characterization of Medicago truncatula root knots induced by Meloidogyne incognita

Guhl, Katherine Elizabeth.

January 2006

Thesis (M.S.)--University of Delaware, 2006. / Principal faculty advisor: Darla J. Sherrier, Dept. of Plant and Soil Science. Includes bibliographical references.

Seleção de caracteres complexos em alfafa por meio de inteligência computacional / Complex traits selection in alfalfa by means of computational intelligence

Santos, Iara Gonçalves dos

18 July 2017

Submitted by Reginaldo Soares de Freitas (reginaldo.freitas@ufv.br) on 2018-01-16T11:32:00Z No. of bitstreams: 1 texto completo.pdf: 1247418 bytes, checksum: e985fa1f1156f534c1dbec006984c2de (MD5) / Made available in DSpace on 2018-01-16T11:32:00Z (GMT). No. of bitstreams: 1 texto completo.pdf: 1247418 bytes, checksum: e985fa1f1156f534c1dbec006984c2de (MD5) Previous issue date: 2017-07-18 / Conselho Nacional de Desenvolvimento Científico e Tecnológico / O desenvolvimento de novos cultivares de alfafa está relacionado, além do potencial produtivo, com o valor nutritivo da forragem, ambos determinados por uma série de caracteres de controle genético complexo. Por isso, o melhoramento da cultura exige adoção de técnicas que maximizem a acurácia seletiva. Nesse contexto, a utilização das Redes Neurais Artificiais (RNAs) pode ser útil para otimizar a seleção simultânea de caracteres, que tem sido a estratégia mais utilizada no melhoramento da alfafa. Assim, o objetivo deste trabalho foi aplicar a abordagem de índices de seleção no contexto das redes neurais artificiais para auxiliar o melhoramento da cultura da alfafa, além de avaliar a eficiência das redes para realizar a seleção de caracteres complexos. Para isso, foram utilizados dados de 77 genótipos de alfafa avaliados em quatro cortes realizados ao longo das diferentes estações no ano, mensurados quanto a caracteres de produção e valor nutritivo. Primeiramente, foram estimados os ganhos por seleção direta, indireta e simultânea pelo índice de Taí para cada um dos grupos de caracteres. Para obtenção das redes para cada grupo, os genótipos foram subdivididos em classes segundo os escores do índice. A fim de garantir boa capacidade de generalização das redes, nas etapas de treinamento e validação foram utilizados dados ampliados de cada grupo de caracteres e, só então, as redes foram utilizadas para classificar os dados reais dos quatro cortes. Posteriormente, utilizou- se dados ampliados de três cortes para treinamento e validação e a rede, então estabelecida, foi empregada em dados reais, relativos a um dos cortes que não participou do processo de ampliação. De modo geral, as seleções diretas proporcionaram ganhos per se satisfatórios para os propósitos do melhoramento, mas sua utilização deve ser bastante criteriosa tendo em vista a existência de correlações desfavoráveis entre alguns caracteres estudados. Já as seleções indiretas apresentaram dificuldades para manter ganhos desejados em todos os caracteres no conjunto de genótipos. Os resultados da seleção simultânea utilizando o índice de Taí proporcionaram distribuição de ganhos mais equilibrada para os conjuntos de caracteres em todos os cortes. No contexto das redes neurais artificiais, as taxas de erros das redes de produção e valor nutritivo foram baixas, evidenciando a grande concordância destas com o índice. Entretanto, a limitação do conjunto de treinamento e teste das RNAs para ampliação de três cortes, levou tanto a altas taxas de erro ou a níveis muito baixos, indicativo de perda da habilidade de generalização. Quando se utilizou as redes no novo corte, as taxas de erro foram altas em todos os cenários. O baixo desempenho obtido pode ser explicado pela discrepância observada entre o conjunto de treinamento e o conjunto de teste. Dessa forma, percebe-se a importância da qualidade do conjunto de dados para treinamento de uma rede eficiente, pois a utilização desta é diretamente relacionada com a disponibilidade de bons exemplos e em grande número. O uso das RNAs será mais difundido à medida que haja mudança no paradigma da experimentação em que as decisões passarão a ser tomadas em bancos de dados, construídos ao longo do tempo de um programa de melhoramento, que constituirão de base para o processamento de dados. / Developing new alfalfa cultivars is related with productive potential besides to the nutritive value of the forage, which are determined by traits of complex genetic control. That is why alfalfa breeding requires adoption of techniques that maximize selective accuracy. In this context, using Artificial Neural Networks (ANNs) can be useful to optimize the simultaneous selection, which has been the strategy most used in alfalfa breeding. Thus, the aim of this work was to apply the selection index approach in the context of artificial neural networks to help in alfalfa breeding, as well as to evaluate the efficiency of the ANNs to perform the complex trait selection. The data from 77 alfalfa genotypes evaluated in four cuts were collected considering different seasons in the year. In each cut were measured production and nutritive value traits. Firstly, we estimated the gains by direct, indirect and simultaneous selection by the Taí index for each trait groups. To obtain the ANN for each group, the genotypes were subdivided into classes according to the index scores. In order to ensure good network generalization, in the training and validation stages we used amplificated data from each group of characters, later we used the ANNs to classify the real data of the four cuts. Subsequently, we used amplificated data from three cuts for training and validation, and the established ANNs were used in a new cut that did not participate in the amplification process. In general, the direct selections provided satisfactory individual gains for the breeding purposes, but their use must be very judicious since the existence of unfavorable correlations between some studied traits. Indirect selections, presented difficulties in maintaining desired gains in all traits in the genotype set. The results of simultaneous selection using the Taí index provided a more balanced distribution gains for the trait sets in all cuts. In the context of the artificial neural networks, the error rates of the production and nutritional value groups were low, evidencing the great agreement of these with the index. However, the limitation of the training set and test of ANNs for data of three cut amplification, led either to high error rates or to very low levels, indicating of loss of the generalization ability. When the networks were used in the new cut, error rates were high in all scenarios. The low performance obtained can be explained by the discrepancy between the training set and the test one. In this way, the importance of the quality of data set for training an efficient network is perceived, since its use is directly related to the availability of good examples and in large numbers. The use of ANNs will be more widespread with a change in the experimentation paradigm in which decisions will be made into databases built over time from a breeding program that will form the basis for data processing.

Alfafa - Melhoramento genético

Medicago sativa

Redes neurais (Computação)

Inteligência artificial

Genética Quantitativa

Rezistence vojtěšky seté (Medicago sativa) a rajčete jedlého (Solanum lycopersicum) vůči původcům bakteriálních chorob

Víchová, Jana

January 2004

Angl. resumé

Cukerné hospodářství rostlin a arbuskulární mykorhizní symbióza / Plant sugar metabolism and arbuscular mycorrhizal symbiosis

Konečný, Jan

January 2017

The study of arbuscular mycorrhizal symbiosis (AMS) - the mutualist relationship between the most of land plants and evolutionary old fungal group Glomeromycota - is becoming a prestigious topic. The prevalence of and extent of physiological action of AMS on plants is very interesting for the plant biology itself, but its importance grows, notably in time of global climate change, frequent soil degradation and ascending exhaustion of mineral fertilizer reserves. Although the flows in AMS of some minerals, like of phosphorus was enlightened, carbon exchange between the symbionts is still poorly understood. In this experimental work, I utilized the boom of molecular and bioinformatic methods in the quest for completely unexplained carbon flows. The organisms used include barrel medic (Medicago truncatula), the model legume for symbiotic relationships, biotic, and abiotic stresses; Rhizophagus irregularis, the widely used fungus for such experimental studies of AMS; and Sinorhizobium meliloti, the nodulating nitrogen-fixing bacterium compatible with the barrel medic. Two variants - mycorrhizal (M+) and non-mycorrhizal (NM) plants were subjected to several levels of analysis. I have checked the variants, did the measurements of phosphorus and nitrogen contents, as well as I probed the plants with...

Plusieurs niveaux de contrôle sont mis en jeu lors de flétrissement bactérien chez la légumineuse modèle Medicago truncatula / Several control levels during the bacterial wilt of the model legume plant Medicago truncatula

Turner, Marie

25 September 2009

Nous présentons l’étude de l’interaction entre la bactérie pathogène racinaire Ralstonia solanacearum et la légumineuse modèle Medicago truncatula. Un pathosystème avec les lignées A17 et F83005.5, respectivement sensible et résistante à la souche GMI1000, a été mis en place avec une procédure d’inoculation sur racines intactes. Ce dispositif expérimental nous a permis de suivre le processus infectieux, de la pénétration de la bactérie par l’extrémité racinaire au développement des symptômes foliaires. L’analyse des étapes précoces de l’interaction a permis de décrire l’apparition de symptômes racinaires qui se mettent en place rapidement après l’infection, que les lignées soient résistantes ou sensibles à la bactérie. Un arrêt de croissance de la racine s'observe dès 24 heures post-inoculation, ainsi qu’une mortalité de l’épiderme de l’extrémité racinaire. Ces phénotypes sont notés suite à des inoculations avec de faibles concentrations bactériennes, et ce sur plusieurs espèces hôtes ou non-hôtes testées. La mise en place des symptômes racinaires est dépendante de l’appareil de sécrétion de type III. Un crible de mutants d’effecteurs de type III de la souche GMI1000, basé sur l’apparition des symptômes racinaires, a permis de montrer que des pools différents d’effecteurs interviennent chez A17 et F83005.5. Chez la lignée sensible A17, deux effecteurs sont principalement impliqués, Gala7 et AvrA. L’étude de la colonisation de cette lignée a montré que le mutant gala7 ne pénètre pas la plante et n’induit pas de symptômes de flétrissement. Le mutant avrA s’est révélé capable d’induire la maladie chez la lignée A17 mais de manière nettement réduite par rapport à la souche sauvage. L’analyse des extrémités racinaires des lignées sensible et résistante infectées par la souche GMI1000 a révélé qu’au niveau des parois de l’endoderme, la présence de lignine est induite de manière plus précoce chez la lignée résistante. Des phénomènes de division cellulaire ont été identifiés autour du cylindre central et semblent également liés à une restriction de la propagation bactérienne. Au niveau du contenu cellulaire, une autofluorescence et une production de ROS semblent liés à une phase nécrotrophe de la bactérie lors de sa propagation dans la zone corticale de l’extrémité racinaire. L’étude de la colonisation bactérienne en s’affranchissant de l’étape de pénétration a révélé que des mécanismes de résistances peuvent intervenir au niveau de collet chez la lignée F83005.5 et lors de la colonisation racinaire des vaisseaux conducteurs suite à une inoculation avec le mutant gala7 / Manquant

Ralstonia solanacearum

Medicago truncatula

Mécanismes de virulence

Effecteurs de type 3

Interaction pathogène

Mécanismes de résistance

Mécanismes de sensibilité

Diseño y validación de herramientas biotecnológicas para la mejora del valor nutricional de la alfalfa (Medicago sativa L.)

Fresquet Corrales, Sandra

29 December 2015

[EN] Alfalfa (Medicago sativa L.), is a forage legume with a significant content of protein, being the most widely cultivated forage around the world. In this species, the protein content decreased during growth processes as well as other resources used by the plant during the flowering process. Alfalfa also contains a lower concentration of condensed tannins or proanthocyanidins (PAs), less than required to remedy the digestive disorder of ruminant livestock causing pasture bloat by production of greenhouse gases as result of the microbial fermentation and the excessive desamination of proteins in the rumen (by-pass effect). These defects on nutrition are reflected in the yield and production of ruminants. Both problematics are difficult to improve by conventional methods. The overall objective of this thesis is to develop molecular tools useful for genetic manipulation of certain traits of agronomic interest in alfalfa, to enhance their nutritional value. At a first step, we have developed an Agrobacterium tumefaciens-mediated transformation protocol via somatic embryogenesis applicable to various genotypes of alfalfa to produce viable embryos in the 50% of the inoculated explants. Chimaeric plants or scapes were almost not detected because most of the transgenic plants contained the T-DNA with all the transgenes incorporated, having thus the indispensable tool to perform the other two objectives. We have isolated two orthologs of the TERMINAL FLOWER 1 (TFL1) gene from alfalfa (MsTFL1c and MsTFL1a). Both genes were constitutively expressed in A. thaliana, and later on in alfalfa, to evaluate their possible use as biotechnological tool for the improvement of the nutritional value of this forage legume, producing a delay in the flowering time and thereby an increase of vegetative development. MsTFL1a performs the same functions as TFL1 in Arabidopsis y its overexpression in this plant produces a remarkable delay of flowering time. In alfalfa, its constitutive expression also produces a delay in flowering. However, this phenotype was not associated to an increase of vegetative growth, being plants of reduced size that appears tied to a limitation in cell proliferation. Moreover, the limitation in cell proliferation was associated with a reduction in the expression levels of certain cell division effector genes, as it is the case of cyclins. Our results support the hypothesis that TFL1-like genes could also participate in signaling pathways that regulate cell differentiation in plants. M. sativa could be a good model to study the possible range of biochemical diversification of these proteins. On the other hand, we have made a multigenic construct in the modular cloning system GoldenBraid 2.0 (35S::Del::Ros1::MtANR::MtLAR). In a first step, it was functionally validated by transient expression in N. benthamiana. In addition, this construct was introduced by stable transformation in two experimental models (A. thaliana and N. tabacum) and later on in M. sativa, where it has been studied the integration capacity and expression levels of the different transgenes. In N. tabacum it has been achieved the activation of both the anthocyanin and PAs biosynthetic pathways. However, it was not able to activate both routes in alfalfa. The TFs Delila and Rosea1 were not able to activate the genes involved in the regulation of these metabolic pathways in alfalfa, or were not sufficient levels of expression of both TFs for this purpose. Therefore, this multigenic construct does not resulted a good biotechnological tool for the activation of PAs biosynthesis in alfalfa. Our results suggest that the mechanisms of transcriptional control of both biosynthetic pathways could be different between plant species, and that additional specific genetic information on the anthocyanin and PAs biosynthesis in legumes is needed to efficiently activate both pathways in this species. / [ES] La alfalfa (Medicago sativa L.), es una leguminosa forrajera con un importante contenido en proteína, siendo la más cultivada a nivel mundial. En esta especie, los contenidos protéicos se ven mermados por los procesos de crecimiento y los recursos utilizados por la planta en el proceso de floración. Además, la alfalfa contiene una concentración de taninos condensados o proantocianidinas (PAs) muy inferior a la requerida para subsanar el desorden digestivo del ganado rumiante que genera hinchamiento por gases de efecto invernadero o meteorismo y la excesiva desaminación de las proteínas en el rumen producida por las fermentaciones de la flora microbiana ruminal. Ambas problemáticas son difíciles de abordar mediante métodos convencionales de mejora. El objetivo general de esta Tesis es desarrollar herramientas moleculares de utilidad para la manipulación genética de determinados caracteres de interés agronómico en la alfalfa, con objeto de incrementar su valor nutricional. Para ello, hemos puesto a punto un protocolo de transformación genética mediada por Agrobacterium tumefaciens vía embriogénes somática aplicable a varios genotipos de alfalfa, que permite la producción de embriones viables capaces de germinar y producir plantas completas en el 50% de los explantes inoculados. Prácticamente no se detectó la presencia de quimeras o escapes ya que la mayoría de las plantas obtenidas contenían el T-DNA con todos los transgenes incorporados, disponiéndose por tanto de la herramienta imprescindible para la realización de los otros dos objetivos. Hemos aislado dos ortólogos del gen TERMINAL FLOWER 1 (TFL1) de alfalfa (MsTFL1c y MsTFL1a). Ambos genes se sobreexpresaron constitutivamente en A. thaliana y después en alfalfa para su posible uso como herramienta biotecnológica para producir un retraso en el tiempo de floración y con ello un posible aumento del desarrollo vegetativo. MsTFL1a extiende la fase vegetativa e inflorescente y retrasa la floración en Arabidopsis. En alfalfa su expresión constitutiva también produce retraso de la floración. Sin embargo, a este fenotipo no se le asocia un incremento del desarrollo vegetativo, presentando las plantas un tamaño más reducido que parece vinculado a una limitación en la proliferación celular. Hemos comprobado que este hecho se asocia a una reducción en los niveles de expresión de determinados genes efectores de la división celular, como es el caso de las ciclinas. Nuestros resultados apoyan la hipótesis de que los genes TFL1-like podrían participar adicionalmente en vías de señalización que regulan la diferenciación celular en plantas. También, hemos realizado una construcción multigénica mediante el sistema de clonaje por módulos GoldenBraid 2.0 (35S::Del::Ros1::MtANR::MtLAR). Se ha validado su funcionalidad mediante expresión transitoria en N. benthamiana y se ha introducido de manera estable en dos modelos experimentales: A. thaliana y N. tabacum, y en M. sativa, donde se ha estudiado su capacidad de integración, así como la de expresión de los transgenes. Hemos comprobado que esta construcción multigénica es capaz de activar la ruta de biosíntesis de antocianinas y de PAs en N. tabacum, pero no fue capaz de activar ambas rutas en alfalfa. Los factores transcripcionales Delila y Rosea1 no fueron capaces de activar los genes implicados en la regulación de ambas vías metabólicas en esta especie, o no fueron suficientes sus niveles de expresión para este fin. Por tanto, esta construcción no es una buena herramienta biotecnológica que procure la activación de la ruta de biosíntesis de PAs en la alfalfa. Nuestros resultados sugieren que los mecanismos de control transcripcional de la biosíntesis de antocianinas y PAs son diferentes entre las distintas especies, y que se necesita información genética adicional específica de la biosíntesis de antocianinas y PAs en leguminosas para poder diseñar eficientemente herrami / [CAT] L'alfals (Medicago sativa L.), és una lleguminosa farratgera amb un important contingut en proteïna, sent la més cultivada a nivell mundial. En aquesta espècie, els continguts proteics es veuen desfavorits amb els processos de creixement i els requeriments utilitzats per la planta en el procés de floració. A més, l'alfals conté una concentració de tanins condensats o proantocianidines (PAs) molt inferior a la requerida per a esmenar el desorde digestiu del bestiar remugant que genera unflament per gasos o meteorisme per la producció de gasos d'efecte hivernacle, i l'excessiva desaminació de les proteïnes en el rumen produïda per les fermentacions de la flora microbiana. Ambdós problemàtiques són difícils d'abordar per mitjà de mètodes convencionals de millora. L'objectiu general d'aquesta Tesi és desenvolupar ferramentes moleculars d'utilitat per a la manipulació genètica de determinats caràcters d'interés agronòmic en l'alfals, a fi d'incrementar el seu valor nutricional. Per a això, hem posat a punt un protocol de transformació mediada per Agrobacterium tumefaciens via embriogènesi somàtica aplicable a diversos genotips d'alfals que permet la producció d'embrions viables capaços de germinar i produir plantes completes en el 50% dels explants inoculats. Pràcticament no es va detectar la presència de fugues, ja que la majoria de les plantes obtingudes contenien el T-DNA amb tots el transgens introduïts, tenint per tant la ferramenta imprescindible per a la realització dels altres dos objectius. Es van aïllar i sobreexpressar constitutivament dos ortòlegs del gen TERMINAL FLOWER 1 (TFL1) d'alfals (MsTFL1c i MsTFL1a) en A. thaliana i en alfals per al seu possible ús com a ferramenta biotecnològica, procurant un retard en el temps de floració i amb això un augment del desenvolupament vegetatiu. MsTFL1a estén la fase vegetativa i inflorescent i retarda la floració en Arabidopsis. En alfals la seua expressió constitutiva també produïx retard de la floració. No obstant això, a aquest fenotip no se li associa un increment del desenvolupament vegetatiu, sent les plantes d'una grandària més reduït que pareix vinculat a una limitació en la proliferació cel·lular. Hem comprovat que la limitació en la proliferació cel·lular s'associa a una reducció en els nivells d'expressió de determinats gens efectors de la divisió cel·lular, com és el cas de les ciclines. Els nostres resultats recolzen la hipòtesi que els gens TFL1-like podrien participar adicionalment en vies de senyalització que regulen la diferenciació cel·lular en plantes. Hem realitzat una construcció multigénica per mitjà del sistema de clonatge per mòduls GoldenBraid 2.0 (35S::Del::Ros1::MtANR::MtLAR). S'ha validat funcionalment per mitjà d'expressió transitòria en N. benthamiana. A més, s'ha introduït de manera estable en dos models experimentals (A. thaliana amb N. tabacum), i finalment en M. sativa, en els que s'ha estudiat la seua capacitat d'integració, així com la d'expressió dels transgens. Hem mostrat que aquesta construcció multigénica és capaç d'activar la ruta de biosíntesi d'antocianines i de PAs en N. tabacum. No obstant això, no van ser capaços d'activar la ruta de biosíntesi d'antocianines i per tant, la de PAs, en alfals. Els factors transcripcionals Delila i Rosea1 no són capaços d'activar els gens implicats en la regulació d'ambdues vies metabòliques en aquesta espècie, o alternativament no van ser prou els seus nivells d'expressió per a este fi. Per tant, aquesta construcció multigénica no és una bona ferramenta biotecnològica per activar la ruta de biosíntesi de PAs en l'alfals. Els nostres resultats suggerixen que els mecanismes de control transcripcional de la biosíntesi d'antocianines i PAs són diferents entre les distintes espècies, i que es necessita informació genètica addicional específica de la biosíntesi d'antocianines i PAs en lleguminoses per a / Fresquet Corrales, S. (2015). Diseño y validación de herramientas biotecnológicas para la mejora del valor nutricional de la alfalfa (Medicago sativa L.) [Tesis doctoral no publicada]. Universitat Politècnica de València. https://doi.org/10.4995/Thesis/10251/59240 / TESIS

Alfalfa

Medicago sativa

Transformación genética

Restraso de la floración

MsTFL1a

MsTFL1c

Síntesis de proantocianidinas

Delila

Rosea1, MtANR

MtLAR