Hibridação somática visando à produção de genitores tetraplóides para o melhoramento de cultivares copa de citros / Somatic hybridization in order to obtain tetraploid parents for citrus scion improvement

Leonardo Soriano

27 January 2011

A hibridação somática via fusão de protoplastos é um método de combinação genética que agrega integralmente os dois genomas genitores, assim como suas respectivas organelas citoplasmáticas, sendo uma ferramenta alternativa aos métodos convencionais de melhoramento. O objetivo deste trabalho foi a obtenção de híbridos somáticos interespecíficos de laranja doce (Citrus sinensis L. Osbeck) \'Pêra\' e \'Westin\' com a tangerina \'Fremont\' (C. clementina hort. ex Tan. x C. reticulata Blanco), \'Thomas\' (C. reticulata Blanco) e \'Nules\' (C. clementina hort. ex Tan), e o tangelo \'Nova\' (C. reticulata Blanco x C. paradisi Macf.) visando à produção de genitores tetraplóides com características agronômicas desejáveis. Como fontes de protoplastos foram utilizados calos embriogênicos de laranja e folhas jovens de tangerina e tangelo, coletadas de plantas cultivadas em casa-de-vegetação. Para o isolamento dos protoplastos, as células de ambas as fontes foram imersas em solução enzimática e incubadas no escuro por 14 horas, sob agitação. Após o isolamento, os protoplastos isolados de calos foram fundidos quimicamente (polietilenoglicol - PEG) com protoplastos não embriogênicos, isolados de mesofilo foliar. Em seguida, os protoplastos foram plaqueados nos meios de cultura líquido BH3, EME e BH3 + EME, e incubados em ausência de luz, sob temperatura de 27 ºC. Após 20 dias de incubação, foram iniciados subcultivos sequenciais para nutrição e redução do potencial osmótico do meio de cultura. Os microcalos desenvolvidos foram transferidos para meio de cultura EME + maltose (13 g.L-1) para a indução da embriogênese somática. Os embriões desenvolvidos foram transferidos para meio de cultura EME + sacarose (25 g.L-1) e em seguida para o meio de cultura 1500 (1,5 g.L-1 de extrato de malte) e finalmente para o meio B+ para desenvolvimento e germinação. As plantas regeneradas foram individualizadas, enraizadas ou microenxertadas e aclimatizadas em casa-devegetação. A confirmação da hibridação somática foi feita por análise morfológica, determinação da ploidia, por citometria de fluxo e análise do DNA com marcadores moleculares do tipo SSR e RAPD. Foram obtidos híbridos somáticos de três combinações (Pêra + Fremont, Pêra + Nules e Pêra + Nova) os quais serão avaliados para utilização diretamente como copa ou como genitor tetraplóide em programas de melhoramento de citros. / Somatic hybridization by protoplasts fusion is a method of genetic combination of two parental genomes, and their cytoplasmic organelles. It is an alternative tool to conventional breeding methods. The objective of this work was to obtain interspecific somatic hybrids of \'Pera\' and \'Westin\' sweet oranges (Citrus sinensis L. Osbeck) with \'Fremont\' (C. clementina hort. ex Tan. x C. reticulata Blanco), \'Thomas\' (C. reticulata Blanco) and \'Nules\' (C. clementina hort. ex Tan) mandarins and Nova tangelo (C. reticulata Blanco x C. paradisi Macf.) to produce tetraploid parents with desirable agronomic characteristics. The sources of protoplasts were sweet orange embryogenic callus and mandarin and tangelo young leaves, collected from plants cultivated in screenhouses. For protoplasts isolation, cells from both sources were immersed in enzyme solution and incubated in the dark for 14 hours (40 rpm). After isolation, the protoplasts isolated from callus were fused chemically (polyethylene glycol - PEG) with non embryogenic protoplasts, isolated from leaf mesophyll. The protoplasts were cultivated in BH3, BH3 + EME and EME liquid culture media and incubated in the dark, under temperature of 27 ºC. After 20 days of incubation, subcultures were initiated in order to reduce the osmotic potential of culture medium. The microcalus developed were transferred to EME medium supplemented with maltose (13 g.L-1) to induce somatic embryogenesis. The developed embryos were transferred into EME + sucrose (25 g.L- 1), culture medium 1500 (1.5 g.L-1 of malt extract) or B+ culture medium for development and germination. The regenerated plants were individually rooted or micrografted, and further acclimatized in screenhouse. Somatic hybridization was confirmed by analysis of leaf morphology, ploidy determination by flow cytometry and molecular analysis by SSR and RAPD markers. Somatic hybrids were obtained of the three combinations (Pera + Fremont, Pêra + Nules and Pêra + Nova) which will be evaluated for direct are as scion or as a tetraploid parent in citrus breeding programs.

Cultura de tecidos vegetais

Embriogênese somática

Frutas cítricas

Hibridação

Melhoramento genético vegetal

Protoplasmos

Citrus

Embriogênese

Genetic plant breeding

Plant tissue culture

Protoplasts.

Somatic embryogenesis

Somatic hybridization

Aspectos fisiológicos, bioquímicos e análise proteômica comparativa durante a maturação, germinação e conversão em plantas de embriões de Ocotea catharinensis Mez. (Lauraceae). / Physiological, biochemical aspects and comparative proteomic during maturation, germination and seedling conversion of Ocotea catharinensis Mez. (Lauraceae).

Leonardo Lucas Carnevalli Dias

16 April 2009

A semelhança entre os eventos da embriogênese zigótica e somática permite que sejam estabelecidos parâmetros para o acompanhamento destes dois processos. Neste trabalho foi estudada a embriogênese somática em Ocotea catharinensis, nas fases de maturação e germinação, além do processo germinativo da semente zigótica, avaliando-se parâmetros bioquímicos, e a expressão diferencial de proteínas. O tratamento com ABA + PEG em culturas de embriões somáticos apresentou variações semelhantes a apresentadas por embriões zigóticos no estádio de maturação. Não se observou a germinação de embriões somáticos, contudo verificou-se que a desidratação prévia promoveu importantes alterações bioquímicas. Durante a germinação, não se observou à síntese de novas proteínas no embrião zigótico. Os estudos proteômicos no desenvolvimento da semente permitiram a seleção de polipeptídios, marcadores estádio-específicos. Os resultados obtidos possibilitam a otimização e melhor entendimento das etapas da embriogênese somática, em espécies com sementes recalcitrantes, como O. catharinensis. / The great similarity among the events of zygotic and somatic embryogenesis allows the establishment of parameters for accompaniment of these processes. In the present work it was studied the somatic embryogenesis in Ocotea catharinensis, in the maturation and germination phases, and the zygotic embryogenesis. The biochemical parameters and differential expression of proteins were evaluated: The treatment with ABA + PEG presented similar variations for zygotic embryos in the maturation stage. The germination was not observed for somatic embryos; however, it was verified that the previous dehydration promoted important biochemical alterations. With relation to the zygotic embryo, throughout the germination process, the synthesis of new proteins was not observed. The proteomic studies carried out throughout seed development, allowed the selection of polypeptides with differential expression. The results obtained open perspectives for the methodology optimization of the somatic embryogenesis, for species with recalcitrant seeds, like O. catharinensis.

Bioquímica de plantas

Biotecnologia vegetal

Cultura de tecidos vegetais

Embriogênese somática

Fisiologia vegetal

Proteômica

Plant biochemistry

Plant biotechnology

Plant physiology

Proteomics

Somatic embryogenesis

Tissue culture plants

Indução e controle da embriogênese somática em Ocotea catharinensis e Ocotea odorifera (Lauraceae). / Induction and control of somatic embryogenesis in the Ocotea catharinensis and Ocotea odorifera (Lauraceae).

Marcelo Bregola Furtado

11 May 2010

O. catharinensis e O. odorifera são árvores originárias da Mata Atlântica. Historicamente estas espécies foram intensamente exploradas e atualmente encontram-se vulneráveis de extinção. A embriogênese somática é uma ferramenta de grande potencial na reprodução de espécies de difícil propagação. No presente trabalho analisou-se o efeito dos meios de cultura MS e WPM e de diferentes de ANA e 2,4-D na indução da embriogênese somática nessas espécies. Em O. catharinensis a combinação WPM + 2,4-D mostrou-se mais efetiva na indução de calos. Resultados mais expressivos foram observados no tratamento WPM + 144µM 2,4-D. Os piores índices de indução foram obtidos no meio MS + 2,4-D. Em O. odorifera não foi utilizado o meio MS. Nesta espécie, mais importante do que o tipo do regulador de crescimento foi sua concentração. Maiores percentuais de calos foram observados em concentrações mais elevadas desses reguladores. WPM + ANA mostrou-se bastante efetivo em O. odorifera, ao contrário do que foi observado em O. catharinensis, onde os resultados foram pouco expressivos. / O. catharinensis and. O. odorifera are originary trees of the brazilian Rain Forest. Historically these species had been intensely explored and are currently considered vulnerable of extintion. Somatic embryogenesis is a tool of great potential in the reproduction of species of difficult propagation. In the present work was analyzed the effect of MS and WPM and different concentrations of ANA and 2,4-D in the iniciation of somatic embryogenesis in this species. In O. catharinensis WPM + 2,4-D revealed more effective in the induction of callus. More expressive results had been observed in the treatment WPM + 144µM 2,4-D. The worse rates of induction had been observed at the combination MS + 2,4-D. In O. odorifera the MS medium was not used. In this specie more important of what the type of the growth regulator was its concentration. Higher rates of callus had been observed at higher concentrations of these regulators. WPM + ANA revealed effective in O. odorifera, in contrast of what was observed in O. catharinensis, where the results had been little expressive.

O. catharinensis

O. odorifera

Biotecnologia

Cultura de tecidos vegetais

Embriogênese somática

Reguladores de crescimento vegetal

O. catharinensis

O. odorifera

Biotechnology

Plant growth regulators

Plant tissue culture

Somatic embryogenesis

Strukturální studie proliferační fáze somatické embryogeneze smrku ztepilého pod vlivem aromatických cytokininů / Structural sudy of prolifareation phase of somatic embryogenesis of Norway spruce under the effect of aromatic cytokinines

Kadlecová, Marie

January 2013

Somatic embryogenesis (SE) represents potentially very suitable way of plant production - micropropagation - of plants in vitro. The process had been studied for more than thirty years and a lot of knowledge has been gained in the field though new ways based on new knowledge leading to improvement and increase of the effectiveness of cultivation protocols are still under focus in the field. Relatively recent discovery of aromatic cytokinins lead to new knowledge on very positive effects on different morphogenetic and physiological processes during both cultivation in vitro or in vivo treatments. This gave origin to the topic of the present thesis, which focused on study of the effect of meta-topolin (mT), aromatic cytokinin, on proliferation phase of SE on structural level of embryogenic lines of Norway spruce Picea abies (L.) Karst. The aim of the thesis is analysis of structural development of embryogenic lines with the use of anatomical preparations and quantitative stereological methods. The material represented three embryogenic lines: 107 and 34C were obtained from the Forestry and Game Management Research Institute from the lab of Dr. Jana Malá and the line AFO 541, which was used as a standard line. To compare the effect of mT with benzylaminopurine (BAP) on proportion of different...

Tissue Culture, Genetic Transformation and Cold Tolerance Mechanisms in Cold-Hardy Palms

Lokuge, Meepa A.

08 December 2006

No description available.

Cold-hardy palms

regeneration

somatic embryogenesis

genetic transformation

supercooling

proteomics

cabbage palm, (Sabal palmetto)

needle palm (Rhapidophyllum hystrix)

Transient Expression of BABY BOOM, WUSCHEL, and SHOOT MERISTEMLESS from Virus-Based Vectors in Cotton Explants: Can We Accelerate Somatic Embryogenesis to Improve Transformation Efficiency?

Alejos, Marcos

12 1900

Upland cotton (Gossypium hirsutum L.) is the world's most prominent fiber crop. Cotton transformation is labor intensive and time consuming, taking 12 to 18 months for rooted T0 plants. One rate limiting step is the necessary production of somatic embryos. In other recalcitrant species, ectopic expression of three genes were shown to promote somatic embryogenesis: WUSCHEL (WUS), SHOOT MERISTEMLESS (STM), and BABY BOOM (BBM). WUS is responsible for maintaining stem-cell fate in shoot and floral meristems. STM is needed to establish and maintain shoot meristems. STM and WUS have similar functions but work in different pathways; overexpression of both together converts somatic cells to meristematic and embryogenic fate. BBM encodes an AP2/ERF transcription factor that is expressed during embryogenesis and ectopic expression of BBM reprograms vegetative tissues to embryonic growth. In prior studies, these genes were constitutively expressed, and cultures did not progress beyond embryogenesis because the embryogenic signal was not turned off. In our study, we set out to use these genes to increase the efficiency of cotton transformation and decrease the time it takes to regenerate a plant. A disarmed cotton leaf crumple virus (dCLCrV) vector delivers WUS, STM, or BBM into cotton tissue cultures through Agrobacterium tumefaciens infection. We propose that virus delivery of embryo-inducing genes is a better approach for transformation because A) inserts more than 800 nucleotides are unstable, and will spontaneously inactivate, B) virus DNA can migrate through plasmodesmata to cells around the infected cell, creating a gradient of embryonic potential, C) the virus DNA does not pass through the germ line and the seed will not contain virus. We propose this method of inducing embryogenesis will facilitate the stable transformation of cotton and will be beneficial to the cotton industry. Ectopic expression of AtBBM, AtSTM, and AtWUS GrWUS:meGFP from a constitutive CaMV 35S promoter produced plants with phenotypes similar to those described in previous studies overexpressing AtBBM, indicating that the AtBBM gene was functional. The cotton cotyledon infiltration of the pART27 constructs showed transformed cells in Coker 312 by GFP localization in the nucleus. Although GFP was detected, no visible embryos appeared from the cotyledon. Cotyledons infiltrated with Agrobacterium harboring overexpression vectors withered and aborted after ~2 weeks. The virus-based vector in tissue culture failed to increase transformation efficiency, resulting in no embryos. The combination of hormone concentration showed no contribution to increasing the transformation efficiency.

Wild type

BABY BOOM

SHOOT MERISTEMLESS

WUSCHEL

PCR

pJRT.Agro.CLCrV

Virus binary vector

Somatic Embryogenesis

days post inoculation

Selenium redox cycling; isolation and characterization of a stimulatory component from tissue of loblolly pine for multiplication of somatic embryos; development of an assay to measure l-phenylalanine concentration in blood plasma

DeSilva, Veronica

25 June 2007

Exogenously supplied organoselenium compounds, capable of propagating a selenium redox cycle, were shown to supplement natural cellular defenses against oxidants generated during biological activity. Phenylaminoalkyl selenides were developed in our laboratory as novel substrate analogs for the enzyme dopamine beta-monooxygenase. Recently, phenylaminoalkyl selenides were found to protect plasmid DNA and Molecular beacons from oxoperoxynitrate – mediated damage by scavenging this oxidant and forming the corresponding selenoxides as the sole selenium – containing products. Rate constants were determined for the reactions of the phenylaminoalkyl selenoxides with GSH at physiological pH and 25 degrees C. The kinetic data obtained in current and previous research was subsequently used in a MatLab simulation, which showed the feasibility of selenium redox cycling by GSH in the presence of a cellular oxidant, oxoperoxynitrate. Loblolly pine (LP, Pinus taeda) is the primary commercial species in southern forests covering 11.7 million hectares. Somatic embryogenesis (SE) is an effective technique to implement production of high value genotypes of LP. SE is a multi-step process, which includes initiation of somatic embryo (SME) growth from tree tissue, maintenance and multiplication of early stage SMEs and the maturation / germination phase. In this work, we isolated a substance from stage 2 or 3 LP female gametophyte (FG) tissue that stimulates early stage SME growth, and characterized this substance as citric acid on the basis of 1H NMR and mass spectrometry. We then demonstrated that topical application of citric acid to SMEs stimulates embryo colony growth at p = 0.05 for 3 of the 5 genotypes tested. Phenylketonuria (PKU) is an autosomal recessive disorder caused by an impaired conversion of L-phenylalanine (L-Phe) to L-tyrosine (L-Tyr). A novel assay based on enzymatic - colorimetric methodology (ECA) was developed in order to detect elevated concentrations of L-Phe in undeproteinized plasma of PKU patients via continuous spectrophotometric detection. We report here that L-Phe concentrations in undeproteinized plasma measured using our ECA were comparable to those determined on an amino acid analyzer based on Pearson correlation coefficients and a Bland and Altman comparison.

Phenylalanine dehydrogenase

PMS

MTS

Phenylketonuria

Enzymatic colorimetric assay

Citric acid

Loblolly pine

Somatic embryogenesis

GSH

Recycling

Molecular beacon

Phenylaminoalkyl selenides

Plasma amino acid analysis

HPLC

Tandem mass spectrometry

Peroxynitrite

Oxoperoxynitrate

Phenylaminoalkylselenoxides

Comparison

L-phenylalanine

Selenium

Oxidation-reduction reaction

Loblolly pine

Somatic embryogenesis

Phenylalanine

Blood plasma

Production de protéines recombinantes par des plantes carnivores génétiquement transformées : application à Drosera rotundifolia et transfert de la technologie à Nepenthes alata / Production of recombinant proteins by genetically modified carnivorous plants : application to Drosera rotundifolia and technology transfer to Nepenthes alata

Biteau, Flore

14 May 2009

Le travail présenté porte sur le développement d’une nouvelle technologie innovante, nommée PAT Friday®, visant à produire des protéines recombinantes au sein des sécrétions extracellulaires de plantes carnivores génétiquement modifiées. Deux objectifs ont été fixés : Réaliser la preuve de concept de la technologie sur le modèle expérimental Drosera rotundifolia, en transformant la plante avec des gènes marqueurs et humains afin de mettre en évidence la présence des protéines recombinantes dans la glu ; et développer, après évaluation, la technologie sur un modèle potentiellement industrialisable, Nepenthes alata. Les résultats ont indiqué la présence des deux protéines marqueurs GFP et GUS dans les tissus et dans la glu de Drosera rotundifolia transformées. Les plantes ont également été transformées génétiquement avec les gènes humains de l’interféron gamma et du facteur intrinsèque. Les protéines recombinantes humaines ont été mises en évidence au sein des tissus végétaux. Le potentiel industriel du modèle Nepenthes alata a ensuite été étudié : 10 à 15 kg de protéines totales par hectare et par an peuvent être produits, grâce notamment à des récoltes successives non destructrices, et la possibilité de contrôler l’activité des protéases digestives naturelles. L’élaboration d’un protocole de régénération de la plante a été entreprise par embryogénèse somatique et organogénèse indirecte, en vue de sa transformation génétique. La technologie PAT Friday®, avec des étapes simplifiées d’extraction et de purification des protéines d’intérêt produites dans le liquide digestif, offre de nouvelles perspectives dans le domaine des protéines thérapeutiques produites à partir de plantes / The present work focuses on the development of a new innovating technology, called PAT Friday®, aiming at producing recombinant proteins into the extra-foliar fluid of modified carnivorous plants. Two objectives were assigned to this work : 1- to realize a proof of concept of the technology on the experimental model Drosera rotundifolia, transformed with marker and human genes, to confirm the occurence of the recombinant proteins into glu ; and 2 - to evaluate and develop, the technology on the model Nepenthes alata, more adapted to industrial scaling-up. The results indicate the presence of two marker proteins GUS and GFP inside the tissues and into the glu of modified Drosera rotundifolia plants. The same plant species has also been transformed with human gamma interferon and intrinsic factor genes. The corresponding human recombinant proteins have been detected into the plant tissues. Potential industrial scaling-up has been studied with the species Nepenthes alata. The results show a potential productivity of 10 to 15 kg of total proteins per hectare per year, thanks to non-destructive repeated harvests, and possibility to efficiently control the natural proteinase activity. The elaboration of a regeneration protocol has been undertaken through indirect organogenesis and somatic embryogenesis, with a view to transform genetically this plant. PAT Friday® technology, with simplified extraction and purification methods of the proteins of interest targeted into the liquid secretions, opens new perspectives in the field of therapeutical proteins produced in plants

Drosera rotundifolia

Embryogénèse somatique

Organogénèse indirecte

Poils glanduleux

Callogénèse

Nepenthes alata

Plantes carnivores

GFP

GUS

Protéines recombinantes

Secrétions digestives

Interféron gamma

Recombinant protein

Somatic embryogenesis

IIndirect organogenesis

Callogenesis

Carnivorous plants

Drosera rotundifolia

Glandulat tentacles

Pitchers

660.65

Cultura de tecidos e transformação genética de espécies da família Poaceae / Tissue culture and genetic transformation of Poaceae family species

Cabral, Glaucia Barbosa

11 July 2012

Brachiaria é um gênero de forrageiras da família Poaceae que apresenta plantas que se reproduzem por via sexual e assexualmente por apomixia,reprodução por sementes. A apomixia desperta interesse biológico e biotecnológico, pela perspectiva de levar esta característica de clonagem de plantas via sementes, a outras espécies. As cultivares plantadas de B. brizantha cv. Marandu e B. decumbens cv. Basilisk são poliplóides e reproduzem-se por apomixia, enquanto as plantas sexuais são diplóides,o que inviabiliza os cruzamentos, dificultando sobremaneira o melhoramento. A transformação genética é uma estratégia que vem sendo incorporada ao melhoramento genético. A natureza apomítica destasplantas pode permitir a clonagem e estabilidade das plantas transgênicas. Para transformação genética é necessário o desenvolvimento de um método eficiente de regeneraçãoin vitro. B. brizantha é considerada recalcitrante a cultura de tecidos, e métodos eficientes associados com os sistemas de transformação genética ainda não foram descritos na literatura. O arroz (Oryza sativa) é uma Poaceae modelo para estudos de genética inversa, no entanto, cultivares tropicais do grupo japônica são recalcitrantes a transformação genética, como é o caso da cultivar Primavera. O método direto de transformação genética mais amplamente utilizado é a biobalística, e vem sendo aplicado em espécies de monocotiledôneas, uma vez que essas não são hospedeiros naturais de Agrobacterium tumefaciens. No entanto, vários fatores tem sido testados no sentido de favorecer a interação e transferência de genes durante a cocultura para obtenção de transgênicos em diversas espécies de monocotiledôneas. Os objetivos deste estudo foram obter sistemas de regeneração in vitro deB. Brizanthae de arroz cultivar Primavera para transformação genética destas espécies. Em B. brachiaria foram obtidos sistema de micropropagação, organogênese, calos embriogênicos, unidades embriogênicas e suspensões celulares, e para a cultivar Primavera de arroz foram obtidas unidades embriogênicas, que foram caracterizadas morfo-anatomicamente e quanto as condições de indução, multiplicação e regeneração in vitro. Métodos de expressão transiente e estável de genes marcadores foram estabelecidos para B brizantha via biobalística e Agrobacterium tumefaciens. A natureza da transgenia foi confirmada por métodos histoquímico e molecular como PCR e Southern blot. Os sistemas de regeneração e transformação obtidos mostraram-se eficientes e irão contribuir para os estudos da apomixia e introdução de genes de interesse em braquiária / Brachiaria is a genus of Poaceae family forage grass that reproduces by sexual and asexually by apomixis. Apomixis is of biological and biotechnological interest awakened by the prospect of bringing this feature of cloning plants through seed to other species. B. brizantha cv. Marandu and B. decumbens cv. Basilisk are polyploid and reproduce by apomixis, while the sexual plants are diploid, which makes the crosses, greatly hindering the improvement. Genetic transformation is a strategy that is being incorporated into breeding programs. The nature of these apomictic plants may allow the cloning and the stability of transgenic plants. For genetic transformation is necessary to develop an efficient method of in vitro regeneration. B. brizantha is considered recalcitrant to tissue culture, and efficient methods associated with the genetic transformation systems have not been described in the literature. Rice (Oryza sativa) is a Poaceae model for studies of reverse genetics; however, tropical cultivars from japonica group are recalcitrant to genetic transformation, such as Primavera cultivar. Biolistic is the genetic transformation direct method most widely used, and has been applied to species of monocots, since these are not natural hosts of Agrobacterium tumefaciens. However, several factors have been tested in order to promote interaction and gene transfer during coculture for obtaining transgenics in several monocots species. The objectives of this study were to obtain in vitro regeneration and genetic transformation systems for these species. In B. Brachiaria systemsfor micropropagation, organogenesis, embryogenic units and embryogenic cell suspensions were obtained, and forrice Primavera cultivar embryogenic units were obtained, which was morpho-anatomical characterized and in vitro induction, proliferation and regeneration conditions established. Methods for transient and stable gene expression have been acquired for B. brizanthavia biolistic and Agrobacterium tumefaciens. The nature of the embryogenic callus and transgenic plants was confirmed by histochemical and molecular methods such as PCR and Southern blot. The regeneration and transformation systems showed to be effective and will contribute to apomixis studies and introduction of genes of interest in B. brizantha

Agrobacterium tumefaciens

Agrobacterium tumefaciens

Biobalística

Biolistics

Brachiaria brizantha cv

Brachiaria brizantha cv

Embriogênese somática

Genes marcadores

Marandu

Marandu

Marker genes

Organogênese

Organogenesis

Oryza sativa cv

Oryza sativa cv

Primavera

Primavera

Somatic embryogenesis

Organogênese in vitro e transformação genética de variedades de tangerina (Citrus reticulata Blanco e Citrus clementina hort. ex Tan.) / In vitro organogenesis and genetic transformation of mandarin varieties (Citrus reticulata Blanco e Citrus clementina hort. ex Tan.).

Soriano, Leonardo

10 March 2015

Atualmente, o Huanglongbing (HLB), doença associada à bactéria Candidatus Liberibacter spp., é a principal ameaça dos Citrus, não tendo sido encontrado ainda espécies resistentes e tolerantes. O melhoramento genético tradicional apresenta limitações para a obtenção de novas variedades porta-enxerto e copa de citros em decorrência a fatores ligados à biologia do gênero. Na tentativa de sobrepor essas dificuldades, a transformação genética destaca-se por permitir a introdução de genes exógenos, os quais, além de reduzir o período de obtenção de material melhorado geneticamente, poderão conferir resistência a doenças em variedades de interesse agronômico. Desse modo, o objetivo desta pesquisa consistiu no estudo da organogênese in vitro, e na obtenção de plantas transgênicas via Agrobacterium tumefaciens das tangerinas \'Fremont\', \'Thomas\' e \'Nules\', com o gene que codifica o peptídeo antibacteriano atacina A (attA), controlado pelos promotores AtSUC2 e AtPP2, visando a expressão gênica preferencial nos vasos do floema. Adicionalmente, foi avaliada a transformação genética via A. tumefaciens de suspensões celulares de tangerina \'W-Murcott\', de laranja doce \'Hamlin\' e de tangelo \'Page\', e a transformação genética direta via PEG de protoplastos da tangerina \'W-Murcott\', com os fatores de transcrição VvmybA1 e Ruby, dirigidos pelos promotores com expressão preferencial nos tecidos embrionários 6105 e DC3. A eficiência da organogênese in vitro foi influenciada pelo tipo de explante e concentração de BAP. Após os experimentos de transformação genética de segmentos de epicótilo e internodal das tangerinas \'Fremont\', \'Thomas\' e \'Nules\', as plantas regeneradas foram analisadas por PCR, Southern blot e RT-qPCR e confirmadas como transgênicas pela presença e transcrição do gene attA no tecido vascular. A transformação genética de suspensões celulares mostrou-se eficiente com alta produção de antocianina nos embriões somáticos regenerados de tangerina \'W-Murcott\', de laranja doce \'Hamlin\' e de tangelo \'Page\'. A transformação genética direta de protoplastos de tangerina \'W-Murcott\' mostrou-se viável e também foi possível a obtenção de embriões somáticos transgênicos. Os fatores de transcrição VvmybA1 e Ruby se mostraram úteis para detecção visual do material transgênico / Currently, Huanglongbing (HLB), associated to Candidatus Liberibacter spp., is the main threat to the citrus culture. The conventional plant breeding shows limitations to the obtain new varieties of rootstock and scion, due to factors related to the biology of the genus. In attempt to overcome these barriers, genetic engineering is notable for allowing the introduction of foreign genes, which, besides reducing the time to obtain genetically improved material may confer disease resistance in varieties of agronomic interest. Thus, the objective of the research was the study of in vitro organogenesis, and obtain transgenic plants of \'Fremont\', \'Thomas\' and \'Nules\' mandarins via Agrobacterium tumefaciens with the gene encoding the antibacterial peptide attacin A (attA), controlled by the promoters AtSUC2 and AtPP2, aiming to preferential gene expression in phloem. In addition, the genetic transformation of cell suspensions, via A. tumefaciens, of \'W-Murcott\' mandarin, \'Hamlin\' sweet orange and \'Page\' tangelo and the direct genetic transformation, via PEG, of \'W-Murcott\' mandarin protoplasts were evaluated with VvmybA1 and Ruby transcription factors driven by 6105 and DC3 promoters, with preferential expression in embryonic tissues. The in vitro organogenesis of the varieties studied was influenced by the type of explant and BAP concentration. After genetic transformation experiments of epicotyl and internodal segments of \'Fremont\', \'Thomas\' and \'Nules mandarins, regenerated plants were analyzed by PCR, Southern blot and RT-qPCR and confirmed as transgenic by presence and transcription of attA gene. The genetic transformation of cell suspensions was efficient with high anthocyanin production in the somatic embryos regenerated of \'W-Murcott\' mandarin, \'Hamlin\' sweet orange and \'Page\' tangelo. The direct genetic transformation of \'W-Murcott\' mandarin protoplasts revealed to be viable and it was also possible to obtain transgenic somatic embryos. The VvmybA1 and Ruby transcription factors were useful tools for visual detection of transgenic material

Citricultura

Citrus production

Cultura de tecidos de plantas

Embriogênese somática

Expressão gênica

Gene expression

Genética molecular vegetal

Greening (Doença de planta)

Greening (Plant disease)

Plant molecular genetics

Plant tissue culture

Protoplastos

Protoplasts

Somatic embryogenesis