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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
91

Controle do desenvolvimento vegetal pela interação auxina-citocinina. Uma nova abordagem baseada no estudo de mutantes de tomateiro (Solanun lycopersicum cv Micro-Tom) / Control of plant development by auxin-cytokinin interactions. A new approach based on tomato (Solanum lycopersicum cv Micro-Tom) mutants.

Pino-Nunes, Lilian Ellen 23 June 2009 (has links)
Os hormônios auxina e citocininas são essenciais ao desenvolvimento das plantas, pois controlam os processos de divisão, expansão e diferenciação celular, os quais, por sua vez, influenciam desde a formação do embrião até o amadurecimento dos frutos e senescência. Auxinas e citocininas regulam respostas fisiológicas comuns, sugerindo haver múltiplos mecanismos de interação. Neste trabalho, um modelo para estudar a interação entre auxinas e citocininas no controle do desenvolvimento é proposto, sendo baseado em plantas mutantes e transgênicas, além de duplos mutantes, com alterações na sensibilidade ou metabolismo de auxina e citocinina. O mutante bushy root (brt) foi caracterizado como pouco sensível à citocinina e sugere uma importante função da citocinina no desenvolvimento da semente e na determinação da dominância apical em tomateiro. Os mutantes potato leaf (c) e entire (e) foram introgredidos no background Micro-Tom (MT), caracterizados e utilizados para verificar como eles afetam a sensibilidade à auxina e como interferem no desenvolvimento da planta. Esses mutantes foram comparados com MT, com o mutante diageotropica (dgt), que é pouco sensível à auxina, e com os duplos mutantes c dgt e dgt e. A mutação c não alterou a sensibilidade à auxina e estaria influenciando apenas a arquitetura foliar. O mutante e parece ser mais sensível à auxina com relação à capacidade de formar raízes in vitro e partenocarpia. O duplo mutante dgt e mostrou fenótipo aditivo (intermediário), sugerindo que DGT e E agem em vias paralelas na resposta à auxina. Foram criadas linhagens transgênicas com superexpressão da enzima citocinina oxidase de Arabidopsis (35S:AtCKX2), que resulta em plantas com baixos níveis endógenos de citocinina. As linhagens transgênicas (MT CKX2 e dgt CKX2) foram comparadas com MT, brt, dgt e brt dgt. A maioria dos parâmetros que estavam relacionados com o desenvolvimento vegetativo, e todos os parâmetros relacionados ao desenvolvimento reprodutivo, foram associados ao efeito dos níveis absolutos de auxina e citocinina, sendo provavelmente resultantes de alterações nos processos de divisão e expansão celular. A dominância apical e a morfogênese in vitro (formação de gemas caulinares e raízes) foram associadas ao efeito do balanço auxina/citocinina, sendo esses processos conhecidamente regulados pelo efeito dessas classes hormonais na diferenciação celular / The plant hormones auxin and cytokinin are crucial for plant development, since they control cell division, expansion and differentiation, which regulate developmental processes starting from embryo formation to fruit ripening and senescence. Auxins and cytokinins usually regulate the same physiological responses, suggesting multiple mechanisms of interaction between these hormones. In this work, a model to study auxin and cytokinin interaction in the control of plant development is proposed, based on mutants, transgenic lines and double mutants with alterations on the auxin and cytokinin sensitivity or metabolism. The bushy root (brt) mutant was characterized as having low cytokinin sensitivity and suggested a relevant function to cytokinin in the seed development and apical dominance in tomato. The potato leaf (c) and entire (e) mutants were introgressed in the Micro-Tom background, characterized and used to check how they affect the auxin sensitivity and the plant development. The responses from these mutants were compared to MT and diageotropica (dgt), which is a low sensitive auxin mutant, and also compared to c dgt and dgt e double mutants. The c mutation did not alter the auxin sensitivity and was only related to leaf architecture. The e mutant seemed to be more sensitive to auxin in the in vitro root induction and parthenocarpy. The double mutant dgt e showed an additive phenotype, suggesting that DGT and E act in parallel pathways controlling auxin sensitivity. Transgenic lines were generated overexpressing the cytokinin oxidase from Arabidopsis (35S:AtCKX2), which renders plants with low endogenous cytokinin levels. Transgenic lines (MT CKX2 and dgt CKX2) were compared to MT, brt, dgt and brt dgt. Most of the traits related to vegetative development and all traits related to reproductive development were linked to the effect of auxin and cytokinin absolute levels, probably reflecting to the effect of these hormones in cell division and expansion. Apical dominance and in vitro morphogenesis (shoot and root formation) were linked to the auxin-to-cytokinin ratio, since these processes are well known to be regulated by the effect of these two hormones in cell differentiation
92

Genômica funcional da interação cacaueiro (Theobroma cacao L.) x Moniliophthora perniciosa por meio do sistema modelo Micro-Tom (Solanum lycopersicum L.) / Functional genomics of the interaction cocoa (Theobroma cacao L.) x Moniliophthora perniciosa by means of the model system Micro-Tom (Solanum lycopersicum L)

Scotton, Danielle Camargo 21 September 2012 (has links)
A cultura do cacaueiro (Theobroma cacao L.) na região sul da Bahia foi dizimada com a introdução do fungo Moniliophthora perniciosa. Novas fontes de resistência têm sido buscadas e alternativas são necessárias para assegurar a produção de cultivares considerando a variabilidade genética do patógeno. A descoberta de genes de resistência e de defesa presumíveis a partir de abordagens genômicas impõe a necessidade de estabelecimento de uma plataforma de análise funcional para comprovar a função dos genes identificados e/ou esclarecimento dos mecanismos envolvidos; isto requer o desenvolvimento de métodos de manipulação e/ou inserção de genes, permitindo a superexpressão ou silenciamento de genes de interesse. Os primeiros cacaueiros transgênicos só foram desenvolvidos a poucos anos, e a eficiência do processo ainda é limitada. Há grande influência genotípica na capacidade embriogênica, que reduz a eficiência de obtenção de transgênicos. Micro-Tom tem sido considerado um modelo para pesquisas em tomateiro, sendo uma cultivar miniatura, ciclo de vida curto, porte reduzido e de fácil transformação. MT pode ser usada no estudo da interação com o fungo M. perniciosa, visto a disponibilidade de isolados do biótipo-S que infectam o tomateiro, assim disponibilizando informações dos mecanismos de defesa do T. cacao a M. perniciosa em um menor tempo, suprindo alguns obstáculos encontrados nas características biológicas do cacaueiro. Considerando que durante a patogênese do cacaueiro, M. perniciosa é capaz de desencadear a morte celular programada no tecido infectado, foi analisada a hipótese de que a expressão de genes anti-apoptóticos diminuiria ou minimizaria os efeitos da infecção, permitindo uma menor susceptibilidade. Para tal, foi clonado o gene da proteína Bax-inhibitor-1, que atua como atenuador basal para a progressão da morte celular, e desenvolvida uma construção. Esse gene havia sido detectado numa biblioteca da interação M. perniciosa x T. cacao e identificado com sequência completa, e foi re-introduzido em tomateiro e cacaueiro sob controle de promotor constitutivo. Para o modelo genético MT, plantas transgênicas contendo Bax-inhibitor-1, SKP1 e Cafeína sintase foram obtidas. Plantas transgênicas de tomateiro contendo o gene Bax-inhibitor-1 foram inoculadas com M. perniciosa e demonstraram redução no número de plantas sintomáticas (40%), quando comparadas as plantas de MT inoculadas com o mesmo patógeno (83%). Esses dados corroboram com resultados das inoculações com os fungos necrotróficos B. cinerea, S. sclerotium e S. rolfsii, sendo que as plantas transgênicas inoculadas também apresentaram contenção dos sintomas dessas doenças, uma redução de 40% da área de infecção em comparação as plantas de MT infectadas. Desse modo, pode-se concluir que o gene Bax-inhibitor-1 em MT agiu de forma basal na atenuação da progressão da morte celular, reduzindo os sintomas da vassoura-de-bruxa, da mesma forma que esse transgene contribuiu na redução dos sintomas do mofo cinza, mofo branco e murcha-de-esclerócio, por conter o crescimento e desenvolvimento dos fungos inoculados em tomateiro. Foi possível otimizar o protocolo de embriogênese somática e de transformação genética de cacaueiro, o que levou a obtenção de plantas transgênicas contendo a construção Bax-inhibitor-1, confirmadas por RTqPCR. Indicando que a abordagem de transformação de cacaueiro está implementada no laboratório, porém a baixa eficiência do processo e o tempo necessário ainda impedem seu uso em larga escala para análise funcional / The cultivation of cocoa (Theobroma cacao L.) in south Bahia was decimated by the introduction of the fungus Moniliophthora perniciosa. New sources of resistance have been sought and alternatives are needed to ensure the production of cultivars considering the genetic variability of the pathogen. The discovery of genes for resistance and defense presumed from genomic approaches makes it necessary the establishment of a platform to verify the function of identified genes and/or the elucidation of the mechanisms involved; this requires the development of methods for manipulating and/or insertion of genes, allowing overexpressing or silencing of genes of interest. The first transgenic cocoa were only developed a few years ago, and the efficiency of the process is still limited. There is an expressive influence of the embryogenic capacity, which reduces the efficiency of obtaining transgenic plants. The cultivar Micro-Tom (MT) is considered a model for research on tomato, since it has a miniature size, short life cycle, and facile genetic transformation. MT can be used to study the interaction with the fungus M. perniciosa, since isolates of biotype-S are able to infect tomato, thus provinding inferences about defense mechanisms of T. cacao to M. perniciosa in a short time, providing some obstacles encountered in biological characteristics of cocoa. Since during the pathogenesis of cocoa, M. perniciosa is able to trigger programmed cell death in infected tissue, it was analyzed the hypothesis that the expression of anti-apoptotic genes diminish or minimize the effects of infection, allowing less susceptibility. To this end, was cloned the protein Bax-inhibitor-1, which acts as a basal attenuator for the progression of cell death, was cloned engineered in a vector for genetic transformation. This gene was detected in a library of interaction M. perniciosa x T. cacao and identified with the complete sequence, and was re-introduced into tomato and cocoa under the control of a constitutive promoter. For the genetic model MT, transgenic plants containing Bax-inhibitor-1, SKP1 and Caffeine synthase were obtained. Transgenic tomato plants containing the gene Bax-inhibitor-1 were inoculated with M. perniciosa and demonstrated a reduction in the number of symptomatic plants (40%) compared MT plants inoculated with the same pathogen (83%). These data corroborate results of inoculations with the necrotroph fungi B. cinerea, S. sclerotium e S. rolfsii. Thus, when transgenic plants were inoculated, it was observed a reduction of 40% in the area of infection, compared to infected MT plants. Taken together, the results indicate that the gene Bax-inhibitor-1 acted in the basal attenuation of progression of cell death in MT, reducing the symptoms of the witches\' broom disease, as well as the symptoms of gray mold, white mold and wilt esclerotia. Moreover it was possible to optimize the protocol for somatic embryogenesis and genetic transformation of cocoa, which led to the production of transgenic plants containing the construct Baxinhibitor- 1, confirmed by RT-qPCR. Although, a protocol for cocoa transformation was implemented in the laboratory, its the low efficiency and the time required still prevent its widespread use for functional analysis
93

Transformação genética cloroplastidial visando aumento da eficiência fotossintética em tabaco (Nicotiana tabacum) / The genetic transformation of chloroplast seeking to increase the photosynthesis efficiency in tobacco (Nicotiana tabacum)

Barboza, André Luiz 11 July 2016 (has links)
Ribulose-1,5-Bifsfosfato (RuBP) carboxilase/oxigenase (RuBisCO) é a enzima chave para a fixação do carbono atmosférico e para a produtividade das plantas. Não há, até o momento, uma metodologia estabelecida para otimizar o processo de fixação do CO2 nas diferentes espécies de plantas. Entretanto, a disponibilidade de um protocolo de transformação genética de cloroplasto de tabaco permite tentativas de manipulação da enzima RuBisCO visando aumento da eficiência fotossintética. Nas plantas, esta proteína é formada por 8 subunidades menores codificadas pelo gene rbcS localizado no genoma nuclear e por 8 subunidades maiores codificadas pelo gene rbcL localizado no genoma de cloroplastos. Neste trabalho, dois genes rbcL-sintéticos, um com a substituição da alanina (A) 378 por uma valina (V) (A378V) e outro sem a substituição foram utilizados para a construção dos vetores pTT629, pTT630, pTT632 e pTT633. Estes vetores foram usados para transformar o cloroplasto de folhas de tabaco, pelo método de biolística. Um total de 35 plantas transplastômicas se desenvolveram sob seleção dos antibióticos espectinomicina (500 mg/L) e estreptomicina (500 mg/L) e a análise molecular dos sítios de restrição AccI, EcoRI, NdeI e NsiI, de fragmentos amplificados da sequência codante atpB::rbcL:: aadA:: accD demonstrou a integração dos genes rbcL-sintéticos em 11 linhagens transplastômicas. Sementes F1 destas plantas demonstraram ser homoplásmicas pela germinação na presença do antibiótico espectinomicina (500 mg/L). Análises fisiológicas das taxas de fotossíntese (A), condutância estomática (gs) e de transpiração (E) das plantas transplastômicas (A378V) mantidas em casa-de-vegetação produziram valores maiores e significativos, quando comparados com as plantas sem a mutação e controle não transgênicos. O aumento da taxa de fotossíntese das linhagens transplastômicas indicam a possibilidade de aumento da atividade catalítica da RuBisCO. A compreensão da interação fotossintética com a atividade fotorrespiratória poderá permitir explorar e estender possíveis benefícios, como o aumento da produtividade em cultivares de interesse agronômico. / Ribulose-1,5-Bifsfosfato (RuBP) carboxylase/ oxygenase (RuBisCO) is the key enzyme for the fixation of atmospheric carbon and productivity of plants. At moment, no single solution to optimize the CO2 fixing process by the different species of plants. The availability of a few efficient chloroplast transformation protocols for all cultivars also directs attempts to manipulate the larger and small subunit of RuBisCO. In plants, this protein consists of coding form eight smaller subunits encoding the rbcS gene and 8 larger subunits of the rbcL gene respectively located in the nucleus and chloroplasts. Using two rbcL-synthetic genes, with an alanine (Ala) 378 substituting a valine (Val) (A378V) and another one without the replacement were used in the construction of pTT629, pTT630, pTT632 and pTT633 vectors, which were used in the method of biolistic to driving these transgenes into the chloroplast genome of tobacco. A total of 35 transplastomic plants were grown under selection of antibiotics spectinomycin (500mg/ L) and streptomycin (500mg/ L) and the molecular analysis using restriction sites AccI, EcoRI, NdeI and NsiI from the amplified fragments of atpB::rbcL:: aadA:: accD sequence displayed the rbcL-synthetic genes integrated into the plastome of the 11 transplastomic lines. The F1 seeds of these plants were shown to be homoplasmic from germinating in the presence of the antibiotic spectinomycin (500mg / L). The physiology analyzes of photosynthesis (A), stomatal conductance (gs) and transpiration (E) rates of these transplastomic lines (A378V) plants kept in green-house produced the highest and significant values when when compared to the control plants without the mutation and non-transgenic control. The increase of the photosynthesis rate form transplastomic lines indicates the possibility of increasing the catalytic activity of RuBisCO. The understanding of the photosynthetic interaction with photorespiration activity may allow explore more the potential benefits, such as increased productivity in crops of agronomic interest.
94

Caracterização anatômica da organogênese in vitro e transformação genética via Agrobacterium tumefaciens em Citrus sp. / Anatomical analysis of in vitro organogenesis and Agrobacterium tumefaciens-mediated transformation in Citrus sp.

Almeida, Weliton Antonio Bastos de 28 October 2002 (has links)
A transformação genética vem sendo, cada vez mais, incorporada em programas de melhoramento genético de diversas espécies. Esta técnica permite a incorporação de gene(s) exógeno(s) no genoma das plantas, modificando características específicas. Assim, apresenta-se como uma importante ferramenta de auxílio ao melhoramento convencional de citros, que possui uma série de limitações impostas pela sua biologia reprodutiva. Entretanto, a transformação genética requer o estabelecimento prévio de sistemas de regeneração de plantas in vitro como requisito essencial para sua execução. Portanto, o objetivo deste trabalho foi estabelecer as condições de cultivo in vitro para organogênese e transformação genética de laranja 'Hamlin', laranja 'Pera', laranja 'Valência', laranja 'Natal' (Citrus sinenis L. Osbeck) e limão 'Cravo' (Citrus limonia L. Osbeck), realizando-se a caracterização anatômica do processo. Buscou-se, inicialmente, otimizar o processo de organogênese e regeneração de plantas in vitro, a partir de segmentos de epicótilo. Explantes foram introduzidos em meio de cultura MT suplementado com BAP, nas concentrações 0,0; 0,5; 1,0; 1,5; 2,0; 2,5; 3,0; 3,5; 4,0 ou 4,5 mg.L -1 . Avaliaram-se o percentual de explantes responsivos e o número de brotações maiores ou iguais a 1,0 cm por explante responsivo. As brotações obtidas foram transferidas para meios de enraizamento, que se constituíram do MT + 1,0 mg.L -1 de NAA, MT + 1,0 mg.L -1 de IBA e MT na ausência de auxina. A concentração de BAP que melhor favoreceu a indução da organogênese foi 1,0 mg.L -1 para as laranjas doces e 0,5-2,5 mg.L -1 para o limão 'Cravo'. O meio de enraizamento com melhor resposta foi o MT + 1,0 mg.L -1 de IBA, para todos os cultivares estudados. Procedeu-se análise anatômica da organogênese in vitro, nas condições ótimas obtidas no trabalho anterior. As gemas adventícias tiveram origem endógena, formando-se a partir de zonas meristemáticas do câmbio vascular, caracterizando-se em organogênese direta. Desenvolveram-se, também, experimentos para estudar a transformação genética, via Agrobacterium, em segmentos de epicótilo de laranja 'Natal', laranja 'Valência' e limão 'Cravo'. Neste caso, estudou-se o tempo de inoculação com Agrobacterium, o período de co-cultivo, a utilização de acetoseringona e a temperatura de incubação durante o co-cultivo e o seccionamento do explante. Plantas transgênicas foram obtidas utilizando-se um período de inoculação de 20 minutos com Agrobacterium tumefaciens (EHA-105), co-cultivo por 3 dias na ausência de acetoseringona no meio de cultura e temperatura de co-cultivo de 23-27 °C. Finalmente, desenvolveu-se um estudo da indução da organogênese, análise histológica e transformação genética, a partir de segmentos internodais de plantas adultas das laranjas 'Hamlin', 'Pera', 'Valência' e 'Natal'. A organogênese foi induzida em meio de cultura DBA3, modificado, suplementado com 1,0 mg.L -1 de BAP e 0,5 mg.L -1 de NAA. Em função dos cortes histológicos concluiu-se que as gemas adventícias formaram-se na superfície do calo, o qual originou-se de sucessivas divisões celulares do câmbio, caracterizando-se em organogênese indireta. Plantas transgênicas de tecido adulto de laranja 'Hamlin' e laranja 'Valência' foram obtidas utilizando-se um dia de co-cultivo a 24 ºC, com ou sem o seccionamento do explante para Hamlin e apenas com o seccionamento do explante para Valência. / Genetic transformation has been more frequently associated with conventional genetic breeding programs of different species. It allows for the introduction of exogenous gene(s) into the plant genome, with the possibility of altering specific characteristics. Thus, it can be an important tool for Citrus conventional breeding programs, which present several limitations imposed by the characteristics of the reproductive biology of this genus. For the success of the transformation system, however, the previous establishment of an efficient in vitro regeneration system is required. The objective of this research was to define in vitro culture conditions for the organogenesis and genetic transformation of Hamlin, Pera, Valencia and Natal sweet oranges (Citrus sinensis L. Osbeck) and Rangpur lime (Citrus limonia L. Osbeck) with the anatomical characterization of the process. Initially, the optimization of the in vitro organogenesis process and plant recovery was attempted using epicotyl segments as explants. For organogenesis induction, the explants were placed in MT culture medium supplemented with BAP (0.0; 0.5; 1.0; 1.5; 2.0; 2.5; 3.0; 3.5; 4.0 or 4.5 mg.L -1 ). The percent of responsive explants and the number of adventitious shoots per explant (> 1.0 cm) were evaluated. The shoots were transferred to rooting media, consisting of MT medium supplemented with NAA or IBA, or absence of auxin. The best BAP concentration for organogenesis induction was 1.0 mg.L -1 for the sweet oranges and between 0.5 and 2.5 mg.L -1 for Rangpur lime. The best rooting medium was MT with 1.0 mg.L -1 IBA for all the cultivars. Anatomical analysis was done to describe the optimized culture conditions. Adventitious buds originated endogenously from meristematic regions of the vascular cambium, characterizing a direct organogenesis. Studies were also done to analyze the genetic transformation of the sweet orange cultivars Natal and Valencia and Rangpur lime via Agrobacterium. Several experiments were installed to define the period of Agrobacterium inoculation and co-cultivation, the presence or absence of acetoseryngone, the temperature of incubation and the explant condition (with or without a longitudinal cut). Transgenic plants were obtained using an inoculation period of 20 minutes and co-cultivation for 3 days at 23-27 °C in absence of acetoseryngone in the culture medium. Finally, a study of organogenesis induction, histological characterization and genetic transformation from internodal segments of mature plants of sweet orange cultivars Hamlin, Pera, Valencia and Natal was conducted. Organogenesis was induced in DBA3 modified medium supplemented with 1.0 mg.L -1 BAP and 0.5 mg.L -1 NAA. Histological analysis showed that the adventitious buds formed indirectly from the callus formed by successive cell divisions from the vascular cambium. Transgenic plants from mature tissue of Hamlin and Valencia sweet oranges were obtained using one day of co-cultivation at 24°C with or without the longitudinal sectioning of the explant for Hamlin and only when the explant was longitudinally sectioned for Valencia.
95

Transformação genética de laranja doce com uma construção gênica do tipo hairpin de um fragmento do gene da V-ATPase-A de Diaphorina citri Kuwayama / Sweet orange genetic transformation with a hairpin type construction gene fragment of V-ATPase-A of Diaphorina citri Kuwayama

Silva, Tatiane Loureiro da 12 December 2013 (has links)
O Brasil é o maior produtor de laranja doce no mundo. Entretanto, a cultura enfrenta grandes problemas, devido ao ataque de pragas e doenças, o que reduz a produtividade da cultura. Entre estas doenças, destaca-se o huanglongbing (HLB), doença associada a três espécies da bactéria Candidatus Liberibacter. No Brasil, o psilídeo Diaphorina citri é o inseto transmissor do HLB. A falta de cultivares de laranja doce resistentes ao HLB torna a transformação genética de plantas uma medida em potencial para o controle desta doença. Plantas transgênicas de laranja doce expressando um RNA de dupla fita (dsRNA) de um gene essencial à sobrevivência de D. citri podem resultar no controle do inseto por meio do mecanismo de RNA de interferência. Tal mecanismo resulta na degradação do RNAm homólogo ao dsRNA. Este trabalho teve por objetivo produzir plantas transgênicas de laranja doce, expressando um fragmento do gene DcV-ATPase-A de D. citri, em uma construção gênica tipo hairpin. Dessa forma, o silenciamento gênico por RNA de interferência seria ativado no psilídeo quando este for submetido à alimentação nas plantas transgênicas. O trabalho foi iniciado com a elaboração da construção gênica contendo uma sequência repetida e invertida do gene DcV-ATPase-A de D. citri, para formação de um hairpin. Segmentos de epicótilo, provenientes de sementes germinadas in vitro das laranjas \'Hamlin\', \'Pêra\' e \'Valência\' (Citrus sinensis L. Osbeck) foram utilizados como fontes de explantes para a transformação genética via Agrobacterium tumefaciens. Paralelamente aos experimentos de transformação genética, insetos adultos de D. citri foram submetidos a experimentos de alimentação artificial, contendo RNA de dupla fita (dsRNA) ou pequenos RNA interferentes (siRNA) da DcV-ATPase-A. Ao final do período de alimentação, foram avaliadas o número de insetos vivos e a expressão relativa do RNAm da DcV-ATPase-A. Através de PCR e Southern blot, a transgenia foi confirmada em 26 e 39 plantas de laranja \'Hamlin\' e \'Valência\', respectivamente. A transgenia não foi confirmada nas plantas regeneradas de laranja \'Pêra\'. O número de inserções no transgene variou de 1 a 4 cópias. A produção dos siRNAs foi confirmada em 10 plantas de laranja \'Valência\', através de siRNA blot. O uso de dietas artificiais contendo dsRNA ou siRNA do gene DcV-ATPase-A não resultou em diferenças significativas no número de insetos vivos, ou no nível de expressão relativa do RNAm do gene DcV-ATPase-A em insetos adultos de D. citri. / Brazil is the largest sweet orange producer in the world. However, this crop faces major problems due to the attack of pests and diseases that reduce its productivity. Among the diseases, stands out the huanglongbing (HLB), disease associated with three different species of the Candidatus Liberibacter bacteria. In Brazil, the psyllid Diaphorina citri is the insect vector of HLB. The absence of resistant sweet orange cultivars to HLB makes the genetic transformation of plants a potential methodology to control this disease. Sweet orange transgenic plants engineered to express double strand RNA (dsRNA) of an essential gene for D. citri survival could result in insect control by RNA interference. This mechanism results in degradation of homologous RNAm to dsRNA. The aim of this work was to produce transgenic sweet orange plants expressing a fragment of D. citri DcV-ATPase-A gene, in a hairpin construction aiming gene silencing by RNA interference in D. citri, when fed on sweet orange transgenic plants. The work started developing a gene construct containing an inverted and repeated sequence of DcV-ATPase-A gene, to form a hairpin. Epicotyl segments collected from in vitro germinated seedlings of \'Hamlin\', \'Pêra\' and \'Valência\' sweet oranges (Citrus sinensis L. Osbeck) were used as explants for the genetic transformation experiments via Agrobacterium tumefaciens. At the same time, adults of D. citri underwent artificial diet experiments containing dsRNA or siRNA of DcV-ATPase-A. At the end of feeding time, the survival of insects and the relative expression of DcV-ATPase-A RNAm were evaluated. Through PCR and Southern blot analysis, 26 \'Hamlin\' and 39 \'Valência\' sweet orange transgenic lines were confirmed. None of the regenerated \'Pêra\' plants were transgenic. The transgenic plants had 1 to 4 T-DNA insertions. The siRNA products were observed in 10 \'Valência\' plants, through siRNA blot. The artificial diets containing dsRNA or siRNA of DcV-ATPase-A resulted in no differences in the number of live insects and in the relative expression of DcV-ATPase-A RNAm in adult insects.
96

Isolamento e caracterização de promotores de genes constitutivos de Citrus sinensis / Isolation and characterization of constitutive gene promoters from Citrus sinensis

Lígia Erpen 07 April 2017 (has links)
A transformação genética é uma alternativa ao melhoramento convencional de citros que permite a modificação de genótipos pela introdução de um ou mais genes oriundos de organismos semelhantes ou filogeneticamente distantes do hospedeiro. Os genes transferidos para espécies de interesse devem ser controlados por promotores, os quais regulam a expressão gênica de forma temporal, espacial e na magnitude desejada. Na maioria dos casos, os genes são expressos de forma constitutiva utilizando o promotor CaMV35S isolado do Vírus do Mosaico da Couve Flor. No entanto, o desenvolvimento de novas abordagens de transformação de plantas (cisgenia e intragenia), que fazem o uso de genes e sequências regulatórias derivadas da mesma espécie ou espécies relacionadas, requer a disponibilidade de elementos genéticos, incluindo promotores constitutivos, isolados de citros. Assim, o objetivo do trabalho foi clonar e caracterizar promotores constitutivos de Citrus sinensis. Para isso, a região promotora dos genes Fator de elongação 1-α (CsEF1), Gliceraldeido-3-fosfato-desidrogenase C2 (CsGAPC2) e Cyclofilina (CsCYC) foi isolada e avaliados pela fusão ao gene repórter uidA. A funcionalidade dos três promotores foi confirmada por ensaio histoquímico da atividade GUS em folhas, caules e raízes de plantas transgênicas de citros cv. \'Hamlin\'. A análise de RT-qPCR mostra que a expressão do gene uidA sob controle dos promotores CsCYC, CsGAPC2 e CsEF1 correspondeu a uma atividade aproximada de 64%, 58% e 47%, respectivamente em comparação com o promotor CaMV35S. A análise in silico dos promotores CsGAPC2, CsCYC e CsEF1 mostra que a atividade de cada um é controlada por uma série de putativos elementos cis-regulatórios. A sequência completa e versões truncadas originadas a partir de deleções em cada promotor foram fundidas ao gene uidA e analisadas em plantas transgênicas de Nicotiana benthamiana pelo ensaio histoquímico e fluorimétrico da atividade GUS. As análises de deleções não causaram perda de função dos promotores em estudo, mas afetaram a expressão gênica nos promotores CsGAPC2 e CsEF1. Os promotores isolados representam bons candidatos a serem utilizados em trabalhos de transformação genética de citros. / Genetic transformation is an alternative to citros conventional breeding that allows the modification of genotypes by the introduction of one or more genes derived from different organisms that can not be crossed by natural means. The transferred genes to the species of interest are controlled by promoters, which regulate a gene expression temporally, spatially and in the desired magnitude. In most cases, the introduced genes have been constitutively expressed using the CaMV35S promoter obtained from the cauliflower mosaic virus. However, the development of novel plant transformation approaches (cisgenesis and intragenesis) imply the use of genetic material from the same species or from closely related species capable of sexual hybridization, which requires the isolation of genetic elements, including citros constitutive promoters. The objective of this study was clone and characterize Citrus sinensis constitutive promoters. For this, the promoter region of the genes Elongation Factor 1-α (CsEF1), Glyceraldehyde-3-phosphate dehydrogenase C2 (CsGAPC2) and Cyclofiline (CsCYC) was isolated and evaluated by fusion to the uidA reporter gene. The functionality of three promoter was confirmed by histochemical GUS assay in leaves, stems and roots of transgenic citrus plants cv. \'Hamlin\'. RT-qPCR analysis revealed that uidA gene expression under control of the CsCYC, CsGAPC2 and CsEF1 promoters was approximately 64%, 58% and 47% expression compared with the CaMV35S promoter. In silico analysis of the CsGAPC2, CsCYC and CsEF1 promoters displays their activity is controlled by a series of putative cis-regulatory elements. The full length promoter and truncated versions originated from deletions in promoters sequences were fused to the uidA gene and analyzed in Nicotiana benthamiana transgenic plants by histochemical and fluorimetric GUS assay. Deletion analysis did not cause loss of function on any of the promoters, but affected the gene expression on CsGAPC2 and CsEF1 truncated versions. The isolated promoters represent good candidates to be used in citros genetic transformation.
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Reação à infecção pelo vírus da tristeza dos citros (CTV) em plantas transgênicas de laranja \'Hamlin\' (Citrus sinensis (L.) Osbeck) expressando seqüências gênicas do CTV / Reaction to Citrus tristeza virus (CTV) infection of transgenic \'Hamlin\' sweet orange (Citrus sinensis (L.) Osbeck) plants transformed with CTV genetic sequences

Amancio José de Souza 12 June 2008 (has links)
O vírus da tristeza dos citros (CTV) é uma das maiores ameaças à citricultura mundial. No Brasil, mesmo com a pré-imunização e com a substituição de porta-enxertos, estirpes fortes de CTV ainda causam prejuízos consideráveis. Com o aparecimento da Morte Súbita dos Citros em 1999 e a possível relação desta doença com o CTV, este vírus voltou a figurar como patógeno de importância no cenário da citricultura brasileira. Uma das possíveis soluções para o controle de viroses em fruteiras é a obtenção de plantas transgênicas resistentes ou imunes. O objetivo deste trabalho foi avaliar a resistência ao CTV de plantas transgênicas de laranja \'Hamlin\' contendo três construções gênicas oriundas de seqüências do genoma do CTV. Estas construções gênicas visaram ativar rotas de RNAi (hairpin da capa protéica e seqüência conservada antisenso do CTV) e mecanismos de defesa relacionados à expressão da capa protéica do CTV. As plantas transgênicas foram desafiadas com uma estirpe fraca de CTV (CTV-IAC) por meio de borbulhas e pulgões pretos (Toxoptera citricida Kirkaldy) contendo o vírus. A avaliação da resistênica à replicação viral foi feita por análises de ELISA. As plantas transgênicas foram consideradas não resistentes à infecção e translocação viral quando inoculadas com borbulhas. Entretanto algumas plantas mostraram retardamento da infecção. Não foi possível determinar se houve resistência à transmissão de CTV por pulgões já que a técnica utilizada não foi capaz de infectar os controles de maneira uniforme. / The Citrus tristeza virus (CTV) is one of the greatest threats to the citrus industry worldwide. In Brazil, CTV continues to cause damage through strong strains despite the use of techniques like cross-protection and substitution of intolerant rootstocks. With the appearance and spread of the Citrus Sudden Death disease in 1999 and its possible relation to CTV, this virus was again among important pathogens within the Brazilian citrus industry. One of the possible solutions for controlling virus diseases in fruit crops is the development of immune or resistant transgenic plants. The objective of this work was to evaluate the resistance to CTV of transgenic \'Hamlin\' sweet orange plants containing three transgenic constructs obtained from CTV genomic sequences. The genetic constructs used aimed to activate RNAi defense routes (coat protein hairpin and a conserved sequence from CTV) and resistance mechanisms related to the coat protein expression. The transgenic plants were challenged with a weak strain of CTV, CTV-IAC, by bud and aphid (Toxoptera citricida Kirkaldy) inoculation. The evaluation of viral replication was done by ELISA analysis. The transgenic plants were considered susceptible to viral replication and translocation when bud inoculated. However, a few plants showed retardation of infection. It was not possible to determine resistance in the aphid transmission assay since the controls were not uniformly inoculated.
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Development and application of novel genetic transformation technologies in maize (Zea mays L.)

Ahmad Abadi, Mohammad January 2007 (has links)
Plant genetic engineering approaches are of pivotal importance to both basic and applied research. However, rapid commercialization of genetically engineered crops, especially maize, raises several ecological and environmental concerns largely related to transgene flow via pollination. In most crops, the plastid genome is inherited uniparentally in a maternal manner. Consequently, a trait introduced into the plastid genome would not be transferred to the sexually compatible relatives of the crops via pollination. Thus, beside its several other advantages, plastid transformation provides transgene containment, and therefore, is an environmentally friendly approach for genetic engineering of crop plants. Reliable in vitro regeneration systems allowing repeated rounds of regeneration are of utmost importance to development of plastid transformation technologies in higher plants. While being the world’s major food crops, cereals are among the most difficult-to-handle plants in tissue culture which severely limits genetic engineering approaches. In maize, immature zygotic embryos provide the predominantly used material for establishing regeneration-competent cell or callus cultures for genetic transformation experiments. The procedures involved are demanding, laborious and time consuming and depend on greenhouse facilities. In one part of this work, a novel tissue culture and plant regeneration system was developed that uses maize leaf tissue and thus is independent of zygotic embryos and greenhouse facilities. Also, protocols were established for (i) the efficient induction of regeneration-competent callus from maize leaves in the dark, (ii) inducing highly regenerable callus in the light, and (iii) the use of leaf-derived callus for the generation of stably transformed maize plants. Furthermore, several selection methods were tested for developing a plastid transformation system in maize. However, stable plastid transformed maize plants could not be yet recovered. Possible explanations as well as suggestions for future attempts towards developing plastid transformation in maize are discussed. Nevertheless, these results represent a first essential step towards developing chloroplast transformation technology for maize, a method that requires multiple rounds of plant regeneration and selection to obtain genetically stable transgenic plants. In order to apply the newly developed transformation system towards metabolic engineering of carotenoid biosynthesis, the daffodil phytoene synthase (PSY) gene was integrated into the maize genome. The results illustrate that expression of a recombinant PSY significantly increases carotenoid levels in leaves. The beta-carotene (pro-vitamin A) amounts in leaves of transgenic plants were increased by ~21% in comparison to the wild-type. These results represent evidence for maize to have significant potential to accumulate higher amounts of carotenoids, especially beta-carotene, through transgenic expression of phytoene synthases. Finally, progresses were made towards developing transformation technologies in Peperomia (Piperaceae) by establishing an efficient leaf-based regeneration system. Also, factors determining plastid size and number in Peperomia, whose species display great interspecific variation in chloroplast size and number per cell, were investigated. The results suggest that organelle size and number are regulated in a tissue-specific manner rather than in dependency on the plastid type. Investigating plastid morphology in Peperomia species with giant chloroplasts, plasmatic connections between chloroplasts (stromules) were observed under the light microscope and in the absence of tissue fixation or GFP overexpression demonstrating the relevance of these structures in vivo. Furthermore, bacteria-like microorganisms were discovered within Peperomia cells, suggesting that this genus provides an interesting model not only for studying plastid biology but also for investigating plant-microbe interactions. / Pflanzliche Gentechnik spielt sowohl in der Grundlagenforschung als auch der Biotechnologie eine große Rolle. Allerdings bringt die landwirtschaftliche Nutzung gentechnisch veränderter Pflanzen (GM) ökologische Umweltrisiken mit sich, wie z.B. die Kreuzung GM Pflanzen mit sexuell kompatiblen Verwandten durch Fremdbestäubung. Gegenüber den Kerntransformanden haben Plastidtransformanden für die biotechnologische Nutzung große Vorteile, unter anderem da die Vererbung des Plastidgenoms bei höheren Angiospermen ausschließlich maternal geschieht. Somit kann ein Gentransfer transplastomischer Pflanzen über Pollen ausgeschlossen werden. Zuverlässige in-vitro-Regenerationssysteme, die wiederholte Regenerationsrunden erlauben, sind von großem Wert für die Etablierung der Plastidentransformationstechnologie. Trotz Sein die Hauptgetreidenahrungsmittel der Welt, Zerealie Pflanzen gehören zu schwierigsten in der Gewebekultur zu handeln, die Annäherungen der genetischen Technik streng begrenzt. Im Mais werden hauptsächlich junge zygotische Embryonen für die Herstellung der Regenerations-kompetenten Kalluskulturen benutzt. Der Arbeitsaufwand dafür ist hoch und die Prozedur schwierig und von den Gewächshausbedingungen abhängig. Im Rahmen dieser Arbeit wurden neue Gewebekultursysteme für Mais etabliert, welches junge Blattgewebe nutzt und somit unabhängig von Embryonen und Gewächshaus ist. Weiterhin wurden die aus Blättern gebildeten Kalluskulturen für die Generierung der genetisch veränderten Maispflanzen benutzt. Ebenso wurden verschiedene Selektionsmethoden für die Entwicklung eines Plastidentransformationssystems in Mais getestet. Jedoch konnten keine transplastomischen Maispflanzen erhalten werden. Sowohl die möglichen Ursachen als auch Vorschläge für weiterführende Versuche diesbezüglich werden im Rahmen dieser Arbeit diskutiert. Dennoch stellt diese Arbeit den ersten wesentlichen Schritt für die Entwicklung eines Plastidentransformationssystems in Mais vor. In einem zweiten Teil dieses Projekts wird die erfolgreiche Integration der Narzissen Phytoene Synthase in das Maisgenom durch das neu entwickelte nukleäre Transformationssystem gezeigt. Dadurch konnte eine signifikante Steigerung um 17% des Gesamtcarotinoid- und 21% des Beta-Carotengehalts in Maisblättern beobachtet werden. Schließlich wurden Fortschritte für die Entwicklung eines Transformationssystems für Peperomia (Piperaceae) durch die Etablierung eines Regenerationssystems aus Blättern gemacht. Außerdem wurden Faktoren, die die Plastidengröße und –zahl bestimmen, untersucht. Diese Ergebnisse geben Hinweise darauf, dass die Organellengröße und –zahl eher gewebespezifisch als in Abhängigkeit vom Plastidentyp reguliert wird.
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The regulatory network controlling natural competence for DNA uptake in Vibrio cholerae

Antonova, Elena S. 02 April 2013 (has links)
The bacterial pathogen Vibrio cholerae is responsible for ongoing cholera outbreaks in Haiti and elsewhere. Association of V. cholerae with the human host is responsible for fatal disease, but the bacteria also reside as natural inhabitants of aquatic environments, commonly attaching as biofilms to chitinous surfaces of copepods and crabs. Prior studies in V. cholerae demonstrated that competence for genetic transformation, a mechanism of horizontal gene transfer (HGT), requires the TfoX regulator protein that is triggered by chitin, and the HapR transcription factor that is made in response to quorum sensing (QS) signals produced by V. cholerae and Vibrios. To define regulatory components connecting extracellular signals to natural competence, I first demonstrated that QS molecules produced by Vibrios within multi-species chitinous biofilms are required for DNA uptake by V. cholerae, confirming the critical role of QS signals in HGT. Second, I identified by transposon-mutagenesis a new positive regulator of competence, CytR (cytidine repressor), only studied prior in E. coli as a regulator of nucleoside scavenging. Specific mutations in V. cholerae CytR impaired expression of competence genes and halted DNA uptake; and the addition of exogenous cytidine had similar affects as predicted in E. coli. V. cholerae and other competent Vibrios encode TfoX, HapR, and CytR, although none of these regulators directly controls genes coding for the DNA uptake apparatus. Thus, these results have uncovered a regulatory network, likely used by many Vibrios, that contains additional factors linking several extracellular chemical molecules (cytidine, chitin, and QS signals) to DNA uptake. My study has begun to define a molecular mechanism by which both environment and genetics contribute to genome evolution for this important marine pathogen.
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Regeneration Of Lentil (lens Culinaris Medik) And Genetic Transformation By Using Agrobacterium Tumefaciens-mediated Gene Transfer

Celikkol Akcay, Ufuk 01 April 2008 (has links) (PDF)
In this study, the effects of different plant growth regulators on regeneration responses of various lentil explants through direct and indirect organogenesis and through somatic embryogenesis from calli and cell suspension cultures were investigated. Shoot regeneration was obtained in low frequencies from longitudinal embryonic axis explants and nodal buds of epicotyls, however whole plant regeneration was unsuccessful. Conditions provided for indirect organogenesis resulted only in swelling of hypocotyls and root directed ends of internodes and weak callus formation on leaves which were followed by tissue browning and necrosis. In somatic embryogenesis studies, the explants longitudinal embryonic axis and cotyledonary petioles produced soft and friable calli on MS media with Gamborg&rsquo / s vitamins supplemented with 0.75mg/L 2,4-D+0.5mg/L BA. The highest average number of embryos per explant, 12.36 was observed on media containing 0.75mg/L BA +0.5mg/L 2,4-D for cotyledonary petiole explants, whereas 3mg/L BA+1mg/L NAA was the only hormone combination that allowed embryo development to some extent, in both explants. Somatic callus failed to regenerate despite globular embryo formation and embryo development to some extent. Combination of sonication treatment with Agrobacterium transformation of three lentil explants / cotyledonary nodes, half cotyledons and cotyledonary nodes with intact shoots, had no effect on the improvement of transient gus gene expression on explants. Sonication treatment was also unable to form localized wounds on the petiole axils. The best gus gene expression on the axil region was obtained when cotyledonary nodes and KYRT1 strain were used in combination with vacuum infiltration and scalpel wounding of the axils. Gradual selection and repeated removal of regenerated shoots between selection cycles increased the number of gus expressing shoots significantly. The regenerated shoots were grafted on root stocks and whole plant regeneration was achieved in greenhouse conditions. By the use of the optimized Agrobacterium-mediated transformation protocol, 4 independent lines were obtained with 2.3% transformation efficiency. Southern blot analysis confirmed the integration of the gus gene into the genome of lentil plants. T0 plants were fertile and all plants showed Mendelian segregation of the gus gene in 3:1 ratio to their progenies except one line which carries three copies of the gene. Reverse transcription PCR has confirmed the expression of the genes in T0 and T1 generations. T0 plants and the following three generations strongly expressed gus gene uniformly in their tissues and the PCR amplifications of both gus and npt-II genes was successful through generations.

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