The expression of Dianthin 30, a ribosome inactivating protein

Maree, H. J. (Hans Jacob)

03 1900

Thesis (MSc)--Stellenbosch University, 2003. / ENGLISH ABSTRACT: Ribosome inactivating proteins (RIPs) are currently classified as rRNA N-glycosidases, but also have polynucleotide: adenosine glycosidase activity. RIPs are believed to have anti-viral and anti-fungal properties, but the exact mechanism of these proteins still need to be elucidated.The mechanism of resistance however, appears to be independent of the pathogen. For resistance the RIP terminates virus infected plant cells and stops the reproduction and spread of the virus. Transgenic plants containing RIPs should thus be resistant to a wide range of viruses. The ultimate goal of the larger project of which this forms part is the development of virus resistant plants. To monitor the expression of a RIP in a transgenic plant a detection method had to be developed. Antibody detection of the RIP was decided upon as the most cost effective method. The RIP, Dianthin 30 from Dianthus caryophyllus (carnation), was used and expressed in bacterial and insect expression systems. The bacterial expression experiments were done using the pET expression system in BL21(DE3)pLysS cells. The expression in this system yielded recombinant protein at a very low concentration. Expression experiments were also performed in insect tissue culture with the baculovirus vector BAC-TO-BAC™.With this system the expression was also too low to be used for the production of antibodies. A Dianthin 30 specific peptide was then designed and then produced by Bio-Synthesis. This peptide was then used to raise antibodies to detect Dianthin 30. These antibodies were tested on Dianthus caryophyllus proteins. To establish if this detection method was effective to monitor the expression in plants, tobacco plants were transformed with Agrobacterium tumefaciens containing Dianthin 30 in the pART27 plant expression vector. The putative transformed plants were analysed with peR and Southern blots. / AFRIKAANSE OPSOMMING: Tans word Ribosomale-inaktiverende proteïene (RIPs) geklassifiseer as rRNA N-glikosidase wat ook polinukleotied: adenosien glikosidase aktiwiteit bevat. Daar word geglo dat RIPs anti-virale en anti-fungus eienskappe bevat, maar die meganisme van beskerming word nog nie ten volle verstaan nie. Dit is wel bewys dat die meganisme van weerstand onafhanklik is van die patogeen. Virus geinfekteerde plantselle word deur die RIP gedood om die voortplanting en verspreiding te bekamp en sodoende word weerstand bewerkstellig. Transgeniese plante wat dan 'n RIP bevat sal dus weerstandbiedend wees teen 'n wye spektrum virusse. Die hoofdoel van die breër projek, waarvan die projek deel uitmaak: is die ontwikkeling van virusbestande plante. Om die uitdrukking van die RIP in die transgeniese plante te kontroleer, moes 'n deteksie metode ontwikkel word. Die mees koste effektiewe deteksie metode is met teenliggame. Die RIP, Dianthin 30 from Dianthus caryophyllus (angelier) was gebruik vir uitdrukking in bakteriele- en insekweefselkultuur. Die bakteriele uitdrukkingseksperimente was gedoen met die pET uitdrukkings sisteem III BL21(DE3)pLysS selle. Die uitdrukking in die sisteem het slegs rekombinante proteïene gelewer in uiters lae konsentrasies. Uitdrukkingseksperimente was ook gedoen in insekweefselkultuur met die baculovirus vektor BAC-To- BACTM. Met die sisteem was die uitdrukking ook veels te laag om bruikbaar te wees vir die produksie van teenliggame. Daar is toe 'n peptied ontwerp wat Dianthin 30 kan verteenwoordig vir die produksie van teenliggame. Die teenliggame is getoets teen Dianthus caryophyllus proteïene. Om vas te stel of die deteksiemetode wel die uitdrukking van Dianthin 30 sal kan monitor, is tabak ook getransformeer met Dianthin 30. Die transformasies is gedoen met die hulp van Agrobacterium tumefaciens en die pART27 plant uitdrukkings vektor. Die plante is getoets met die polimerase ketting reaksie en Southern klad tegnieke.

Virus diseases of plants

Plant viruses -- Control

Transgenic plants

Aspectos biológicos de Spodoptera cosmioides Walker, 1858 (Lepidoptera: Noctuidae) nas cultivares de algodoeiro DeltaOPAL e NuOPAL (Bollgard I)

Araújo, Carolina Rodrigues de [UNESP]

17 February 2009

Made available in DSpace on 2014-06-11T19:25:19Z (GMT). No. of bitstreams: 0 Previous issue date: 2009-02-17Bitstream added on 2014-06-13T20:53:02Z : No. of bitstreams: 1 araujo_cr_me_jabo.pdf: 3312351 bytes, checksum: 263e48cc89172f756fb22bf527953bc5 (MD5) / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES) / Spodoptera cosmioides Walker, 1858 é uma espécie polífaga, resistente a inseticidas em várias regiões do país e, apesar de ocorrer em baixas densidades, é considerada uma praga potencial para as culturas de algodão, soja e feijão no cerrado. Neste trabalho, estudou-se a biologia comparada de S. cosmioides sobre a cultivar transgênica comercial NuOPAL (Bollgard I, Evento 531) e sobre a cultivar convencional DeltaOPAL, procurando-se detectar a influência da α -endotoxina CryIAc no desenvolvimento biológico dessa espécie. O experimento foi desenvolvido em condições de laboratório (26 ± 1ºC; UR: 70 ± 10%; fotofase: 12h), a partir de lagartas recém-eclodidas e individualizadas. Foram avaliadas a duração e a viabilidade das fases imaturas, duração do ciclo biológico, peso de pupas, razão sexual, porcentagem de deformação de adultos e de adultos não liberados dos invólucros pupais, longevidade dos adultos, fecundidade e viabilidade de ovos. Os parâmetros biológicos observados não diferiram significativamente em relação às duas variedades. Na cultivar NuOPAL verificou-se maior porcentagem de ovos inviáveis, de adultos deformados e de adultos não emergidos, o que indica que essa cultivar provavelmente afeta a fase adulta de S. cosmioides. / Spodoptera cosmioides Walker, 1858 is a polyphagous species, presents resistance to insecticides in various regions of Brazil, and although it occurs at low densities, it’s considered a potencial pest in the crop of cotton, soybeans and beans in the Brazilian cerrado. In this work was studied the comparative biology of S. cosmioides on the comercial transgenic NuOPAL (Bollgard I, Evento 351) and the conventional cultivar DeltaOPAL to detect the influence of endotoxin-α CryIAc on the biological development of this species. The experiment was conducted under specific conditions in a laboratory (26 ± 1º C; RH: 70 ± 10%; photoperiod: 12h), from newlyhatched and individualized larvae. The duration and viability of immature phases and biological cycle, weight of pupae, sex ratio, percentage of deformed adults and adults not released the pupal beg, longevity of adults, fecundity and viability of eggs were evaluated. The biological parameters observed showed that there weren’t significant difference between two varieties studied. In NuOPAL cultivar there was a greater percentage of eggs unviable, deformed adults and adults not emerged, which indicates that this cultivar probably affects the adult phase of S. cosmioides.

Algodão - Doenças e pragas

Lepdoptero

CrylAc

Gossypium hirsutum

Planta transgênica

Lepidoptera

Transgenic plants

Estudo do papel das proteínas mitocondriais desacopladas na tolerância aos estresses abióticos empregando diferentes abordagens

Nunes, Alessandra Vasconcellos [UNESP]

07 April 2010

Made available in DSpace on 2014-06-11T19:26:02Z (GMT). No. of bitstreams: 0 Previous issue date: 2010-04-07Bitstream added on 2014-06-13T19:53:55Z : No. of bitstreams: 1 nunes_av_me_botib.pdf: 662812 bytes, checksum: e1faf5a1bccf83ade3dc24706edbc278 (MD5) / Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq) / As proteínas desacopladoras pertencem à família de carreadores aniônicos mitocondriais. De maneira geral, as proteínas desacopladoras dissipam o gradiente eletroquímico de prótons gerados na respiração na forma de calor, sendo dependentes de ácidos graxos e sensíveis aos nucleotídeos purínicos. O presente estudo visou investigar o comportamento de plantas transgênicas de tabaco que expressam de forma constitutiva o gene AtUCP1, frente aos estresses osmótico e salino, bem como analisar a atividade das regiões promotoras dos genes AtUCP1 e AtUCP2 de Arabidopsis thaliana, em resposta aos estresses osmótico e de baixa temperatura, e ao ácido abscísico. Numa primeira abordagem foram utilizadas sementes selvagens e de duas linhagens transgênicas, germinadas em meio MS adicionados ou não de NaCl e Manitol. O teste de germinação revelou que as linhagens transgênicas apresentam uma maior tolerância aos referidos estresses. Quando o crescimento radicular foi analisado, uma maior inibição foi constatada no controle não transgênico em relação às duas linhagens transgênicas testadas. Adicionalmente, quando submetidas aos estresses, uma maior acumulação de ânion superóxido foi verificada nas folhas de plântulas não transgênicas em relação às plântulas das linhagens transgênicas. Quanto à quantificação de GUS nas plantas transformadas com os promotores dos genes AtUCP1 e AtUCP2, nenhuma alteração significativa foi observada em nenhum dos tratamentos testados / The uncoupling proteins belong to the mitochondrial anion carrier family. In general, the uncoupling proteins dissipate the proton electrochemical gradient generated in respiration as heat, being dependent on fatty acids and sensitive to purine nucleotides. In the present study, we investigated the behavior of transgenic tobacco plants that overexpress the AtUCP1 gene when subjected to osmotic and saline stress, as well as the activity of the promoters of the AtUCP1 and AtUCP2 genes of Arabidopsis thaliana, in response to osmotic and cold stress, and abscisic acid. In the first approach, seeds from wild type and two transgenic lines were germinated in MS medium containing (or not) NaCl and mannitol. The germination test showed that the transgenic lines have a higher stress tolerance. When root growth was analyzed, a greater inhibition was observed in non-transgenic control seedlings as compared to seedlings of the two transgenic lines tested. Additionally, when subjected to stress, a greater superoxide anion accumulation was detected in leaves of non-transgenic seedlings as compared to seedlings of transgenic lines. Quantification of GUS activity in the plants transformed with the tested promoters, revealed no treatmentspecific differences

Genetica vegetal

Proteinas - Analise

Alimentos geneticamente modificados

Fumo - Cultivo

Uncoupling proteins

Transgenic plants

RNAi para o controle de Tuta absoluta em tomateiro / RNAi for the control of Tuta absoluta in tomato plants

Roberto de Almeida Camargo

31 January 2014

Desde seu descobrimento, o fenômeno de silenciamento gênico por RNA (RNAi) rapidamente se tornou uma técnica amplamente estudada e utilizada nos mais diversos aspectos da biologia molecular. Uma destas possibilidades é sua aplicação no campo da entomologia agrícola, mais especificamente para o controle de insetos-praga como uma alternativa de alta eficiência, especificidade e com impacto ambiental reduzido. Por meio da geração de plantas transgênicas expressando RNAi para genes essenciais de insetos-praga específicos, a ingestão destas moléculas de RNAi pelo inseto mediante herbivoria pode resultar no silenciamento do respectivo gene, resultando em fenótipos que podem variar entre perda de apetite, infertilidade ou até a morte. Neste contexto, o presente trabalho teve como objetivo provar a viabilidade de aplicação desta técnica para a interação Tomateiro x Tuta absoluta, cultura de grande expressão econômica e social no mercado nacional e internacional e que é amplamente atacada por esta praga, com prejuizos que podem alcançar a ordem dos 100% da produção. Por meio da clonagem de genes ortólogos essenciais descritos na literatura e de genes altamente expressos nos primeiros estádios larvais, após a caracterização transcriptômica em escala do inseto, foram realizados ensaios de alimentação contendo moléculas de dsRNAs que possuíam estes genes como alvo. Também, foi realizado a transformação genética de tomateiro cultivar \"Micro-Tom\" com dois destes genes (V-ATPase A e Arginina kinase) para a realização de ensaios de herbivoria. Com os resultados obtidos nestes experimentos, foram mostradas sólidas evidências da viabilidade da técnica de RNAi para o controle de Tuta absoluta, evidenciado pelo silenciamento gênico específico observado no inseto e consequentemente os efeitos nocivos deste silenciamento. / Since their discovery, the phenomenon of gene silencing by RNA ( RNAi ) has rapidly become a widely studied and used technique in the molecular biological field. One of these possible applications is in the entomology field, more specifically for the control of insect pests, as a high efficiency, specificity and with reduced environmental impact alternative. Through the generation of transgenic plants expressing dsRNA targeting essential insect genes, their ingestion by the insect and consequently the uptake of the silencing RNA, may result in specific gene silencing, resulting in a variety of phenotypes that can range from loss of appetite, infertility to death. In this context, this study aimed to prove the feasibility of this technique to control tomato leaf miner (Tuta absoluta) in tomatoes plant, a major crop worldwide and seriously attacked by this pest, with losses that can reach 100%. For the present work, orthologous genes from successfully cases of insect gene silence described in the literature, was selected together with highly expressed genes in the early larval stages of T. absoluta, chosen after the insect molecular characterization and used in feeding assays with dsRNAs molecules to targeted these genes. Also, genetic transformation of the \"Micro-Tom\" tomato cultivar with two of these genes (V-ATPase and Arginine kinase) was conducted for testing in an herbivore assay. With these two approaches was possible to get solid evidences of the feasibility of the RNAi technique to control this insect, evidenced by specific gene silencing observed and its consequent effect on pest phenotype.

Tuta absoluta

RNAi

Silenciamento gênico

Tomateiro

Transformação genética

Tuta absoluta

Gene silencing

RNAi

Tomato

Transgenic plants

Efeito do milho geneticamente modificado MON810 sobre a comunidade de insetos. / Effect of genetically modified corn MON810 on insect community.

Marina Regina Frizzas

11 April 2003

O milho geneticamente modificado MON810, que expressa a proteína Cry1Ab de Bacillus thuringiensis Berliner, está em fase de avaliação e aprovação para liberação comercial no Brasil. Sendo assim, o objetivo da presente pesquisa foi o de estudar os efeitos de MON810 sobre a entomofauna em Barretos/SP e Ponta Grossa/PR no período de 1999 a 2001. O levantamento de insetos foi realizado por meio de diferentes armadilhas (alçapão, bandeja d'água, cartão adesivo e rede de varredura) e contagem de insetos nas plantas de milho, visando avaliar o efeito do milho MON810 sobre a comunidade de insetos, guildas tróficas e dinâmica populacional das espécies predominantes, incluindo organismos benéficos e pragas não-alvo. A interação tritrófica envolvendo milho MON810, Spodoptera frugiperda (J.E. Smith) e Doru luteipes (Scudder) também foi avaliada no presente trabalho. Adicionalmente, um estudo comparativo da comunidade geral de insetos nas diferentes safras de milho foi realizado com o uso de armadilha luminosa. Os tratamentos avaliados foram o milho geneticamente modificado MON810 (MON), milho convencional com aplicação de inseticidas (CCI) e milho convencional sem aplicação de inseticida (CSI). Foi coletado um total de 957.081 espécimes e 409 diferentes espécies. Baseado na análise faunística e índices de riqueza, diversidade, eqüitabilidade e similaridade, não foram observadas diferenças entre os tratamentos na comunidade de insetos. Estes resultados foram também confirmados com as análises de componentes principais e de Kruskal-Wallis. Não foram observadas diferenças significativas entre os tratamentos quanto à proporção relativa de diferentes guildas tróficas analisadas (predadores, parasitóides, polinizadores, decompositores, sugadores e mastigadores). Também não foi observado efeito do milho MON810 na dinâmica populacional das espécies predominantes de aranhas e insetos de diferentes guildas tróficas, incluindo pragas não-alvo e insetos benéficos (Carabidae, Coccinellidae, Chrysopidae, Hemerobiidae, Syrphidae, Tachinidae e Apidae). Avaliações de S. frugiperda e D. luteipes nas plantas de milho confirmaram a eficiência de MON810 no controle desta praga e a sua não interferência na dinâmica populacional do predador. E finalmente, diferenças significativas foram observadas na comunidade geral de insetos nas diferentes safras avaliadas. Portanto, nenhum efeito do milho MON810 foi detectado no presente estudo sobre a comunidade de insetos. / The genetically modified corn MON810, which expresses the Cry1Ab protein from Bacillus thuringiensis Berliner, is under evaluation and approval for commercial release in Brazil. Therefore, the objective of this research was to study the effect of MON810 on insect community in Barretos/SP and Ponta Grossa/PR from 1999 to 2001. The evaluations were based on insect sampling with the use of different traps (pitfall, color tray, sticky trap and sweep net) and insect counts on corn plants to evaluate the effect of MON810 on insect community, throphic guilds and population dynamics of predominant species, including beneficial organisms and non-target pests. Tritrophic interaction involving the corn MON810, Spodoptera frugiperda (J.E. Smith) and Doru luteipes (Scudder) was also evaluated in this study. Additionally, a comparative study of general insect community in different corn growing seasons was conducted with the use of a light trap. The following treatments were evaluated: genetically modified corn MON810 (MON), conventional corn with insecticide application (CWI) and conventional corn without insecticide application (CWI). A total of 957,081 specimens were collected, distributed among 409 different species. Based on faunistic analysis and indexes of richness, diversity, evenness and similarity, there were no differences in the insect community among treatments. These results were also confirmed by principal component and Kruskal-Wallis analysis. No statistical differences were found among treatments in the relative proportion of different trophic guilds evaluated (predators, parasitoids, pollinators, decomposers, suckers and chewers). There was also no effect of MON810 on population dynamics of predominant species of spiders and insects of different trophic guilds, including non-target pests and beneficial insects (Carabidae, Coccinellidae, Chrysopidae, Hemerobiidae, Syrphidae, Tachinidae and Apidae). Evaluations of S. frugiperda and D. luteipes on corn plants confirmed the efficacy of MON810 in the control of this pest and its no effect on the population dynamics of D. luteipes. And finally, significant differences were found in the general insect community in different corn growing seasons. Therefore, no effect of the corn MON810 was detected in this study on insect community.

biodiversidade

insetos benéficos

insetos nocivos

milho

plantas transgênicas

beneficial insects

biodiversity

corn

harmful insects

transgenic plants

Identification and expression analyses of cystolic glutamine synthetase genes in barley (Hordeum vulgare L.)

Goodall, Andrew James

January 2013

Glutamine synthetase (GS) is a key enzyme in nitrogen (N) assimilation, especially during seed development. This thesis has identified three cytosolic GS isoforms (HvGS1) in barley (Hordeum vulgare L. cv Golden Promise). The quantitation of gene expression, isoform localisation and response to N supply has revealed that each gene plays a non-redundant role in different tissues throughout seedling development. The localisation of HvGS1_1 in vascular cells of different tissues, combined with its abundance in the stem and its response to changes in N supply, indicate that HvGS1_1 is important in N transport and remobilisation. HvGS1_1 is located on chromosome 6H at 72.54 cM, close to the marker HVM074 which is associated with a major quantitative trait locus (QTL) for grain protein content (GPC). HvGS1_1 may be a potential candidate gene to manipulate barley GPC. HvGS1_2 mRNA was localised to the leaf mesophyll cells, in both the cortex and the pericycle of roots and was the dominant HvGS1 isoform in these tissues. HvGS1_2 expression increased in the leaves with an increasing supply of N, suggesting that its role is in the primary assimilation of N. HvGS1_3 was specifically and predominantly localised in the grain, being highly expressed throughout grain development. HvGS1_3 expression increased specifically in the roots of plants grown on high NH₄⁺ suggesting that it has a primary role in grain N assimilation and also in the protection from ammonium toxicity in roots. The expression of the HvGS1 genes is directly correlated with both protein and enzymatic activity, indicating that transcriptional regulation is of prime importance in the control of GS activity in barley. Analysis of 15 different barley cultivars found no correlation between HvGS expression and various desirable attributes. Transgenics which over-express and silence individual HvGS1 isoforms have been produced and confirmed, to analyse for changes in beneficial traits.

633.1

Phytoremediation of Nitrous Oxide: Expression of Nitrous Oxide Reductase from Pseudomonas Stutzeri in Transgenic Plants and Activity thereof

Wan, Shen

January 2012

As the third most important greenhouse gas, nitrous oxide (N2O) is a stable greenhouse gas and also plays a significant role in stratospheric ozone destruction. The primary anthropogenic source of N2O stems from the use of nitrogen in agriculture, with soils being the major contributors. Currently, the annual N2O emissions from this “soil–microbe-plant” system is more than 2.6 Tg (one Tg equals a million metric tons) of N2O-N globally. My doctoral studies aimed to explore innovative strategies for N2O mitigation, in the context of environmental microbiology’s potential contribution to alleviating global warming. The bacterial enzyme nitrous oxide reductase (N2OR), naturally found in some soils, is the only known enzyme capable of catalyzing the final step of the denitrification pathway, conversion of N2O to N2. Therefore, to “scrub” or reduce N2O emissions, bacterial N2OR was heterologously expressed inside the leaves and roots of transgenic plants. Others had previously shown that the functional assembly of the catalytic centres (CuZ) of N2OR is lacking when only nosZ is expressed in other bacterial hosts. There, coexpression of nosZ with nosD, nosF and nosY was found to be necessary for production of the catalytically active holoenzyme. I have generated transgenic tobacco plants expressing the nosZ gene, as well as tobacco plants in which the other four nos genes were coexpressed. More than 100 transgenic tobacco lines, expressing nosZ and nosFLZDY under the control of rolD promoter and d35S promoter, have been analyzed by PCR, RT-PCR and Western blot. The activity of N2OR expressed in transgenic plants, analyzed with the methyl viologen-linked enzyme assay, showed detectable N2O reducing activity. The N2O-reducing patterns observed were similar to that of the positive control purified bacterial N2OR. The data indicated that expressing bacterial N2OR heterologously in plants, without the expression of the accessory Nos proteins, could convert N2O into inert N2. This suggests that atmospheric phytoremediation of N2O by plants harbouring N2OR could be invaluable in efforts to reduce emissions from crop production fields.

Greenhouse gas

Nitrous oxide

Nitrous oxide reductase

Phytoremediation

Transgenic plants

GMO crops

Global warming

Climate change

Exploitation of cell wall glycosidase inhibitors to improve wheat resistance against Fusarium graminearum / Exploitation des inhibiteurs de glycosidases de paroi pour améliorer la résistance du blé contre Fusarium graminearum

Tundo, Silvio

11 June 2015

Dans ce travail, nous avons étudié la contribution que les inhibiteurs de glicosidases ont dans la réponse de défense du blé à Fusarium graminearum. Nous avons démontré que les inhibiteurs de xylanases ont la capacité à la fois de contenir l'activité de dégradation de xylanases sécrétées par l'agent pathogène, et de limiter la possibilité de provoquer nécrose dans les tissus du blé. Nous avons démontré que l’expression de la PvPGIP2 dans la lemme, la paléa, les anthères et le rachis détermine une réduction des symptômes de la fusariose de l’épi, au même niveau de l’expression constitutive de cet inhibiteur. Inversement, l'expression de la PvPGIP2 dans l'endosperme ne détermine pas une réduction des symptômes de la maladie. Cela indique que, lorsque l'agent pathogène a atteint ce tissu, l'activité de polygalacturonases de l'agent pathogène n’est pas indispensable pour la propagation fongique. Enfin, la combinaison des différents inhibiteurs de glicosidases, qui renforcent différentes parties de la paroi cellulaire dans le même génotype, a été efficace pour réduire les symptômes de la fusariose, par rapport aux génotypes qui présentent seulment un type d’inhibiteur. Nous avons démontré cet aspect à travers les plantes qui expriment la PvPGIP2 et le TAXI-III. Au contraire, les génotypes qui expriment la PvPGIP2 et l’AcPMEI n’ont pas montré un effect additif sur la résistance, probablement parce que ils renforcent la même partie de la paroi cellulaire, c’est-à-dire la pectine. / In this work we studied the contribution of glycosidase inhibitors in the defense response of wheat against Fusarium graminearum. We demonstrated that xylanase inhibitors are able to limit both the degrading activity of the xylanases secreted by the pathogen and to limit their ability to induce necrosis in wheat cell suspensions and tissues.We demonstrated that the expression of PvPGIP2 in lemma, palea, anthers and rachis causes a reduction in Fusarium head blight symptoms, at the same level of the constitutive expression of this inhibitor. On the contrary, the expression of PvPGIP2 in the endosperm did not result in a reduction of disease symptoms, suggesting that once the pathogen has reached the endosperm, the activity of polygalacturonases secreted by the pathogen is not essential for the progression of symptoms.The pyramiding of glycosidase inhibitors in the same genotype is effective in reducing FHB symptoms although it depends on the specific combination. Pyramiding of PvPGIP2 and AcPMEI does not enhance further wheat resistance against FHB, possibly because they target the same virulent component secreted by the pathogen, that is PG. Conversely, the pyramiding PvPGIP2 and TAXI-III supports a further improvement of resistance compared to plants carrying only PvPGIP2 or TAXI-III.

Fusarium graminearum

Plantes transgéniques

Inhibiteurs de glycosidases

Xylanases

PvPGIP2

Fusarium graminearum

Transgenic plants

Glycosidase inhibitors

Xylanases

PvPGIP2

Monoclonal Antibody Expression and Novel Purification in Nicotiana benthamiana

Fulton, Andrew Dale

28 June 2011

Over the past few decades researchers and industrial professionals alike have realized the vast potential of monoclonal antibodies to treat diseases ranging from arthritis, immune and infectious diseases to cancer. There are a number of antibodies on the market that constitute a large portion of the biopharmaceutical niche in the drug industry. Blockbuster drugs (selling greater than $1 billion/year), include antibodies such as Avastin (bevacizumab), Herceptin (trastuzumab), Rituxan (rituximab), Humira (adalimumab) and Remicade (infliximab), which are cornerstones in this type of sector. With the cost of development to market approval rising astronomically for a new drug, new ways to produce and process these molecules becomes a paramount objective to ultimately help both patients and drug developers. Plants, such as Nicotiana benthamiana, offer a unique production platform due to their recently found ability to produce large amounts of therapeutic proteins in a quick manner. While production would be simple and cheap, purification would not be due to the presence of toxic compounds in ground plant tissue. The current methods to purify these molecules from plant extract include expensive affinity column steps (Protein A/G) that are difficult to scale-up to bed volumes that would be necessary for this technology. In the following paper, a method to purify a monoclonal antibody by non-Protein A/G resins is accomplished and compared to purification by Protein A. The modified process involved an UF/DF step, a precipitation of native impurities step using a charged polymer, hydrophobic interaction chromatography and hydrophobic charge induction chromatography. The yield of this modified process was 19.0%. This process compared favorably with Protein A due to the fact that even with washing steps including NaCl and Tween-20, the Protein A elution fraction still contained a large portion of host cell impurities. A chromatography step would need to be included before Protein A to both protect the column resin and provide a more purified immunoglobulin. / Master of Science

Ebola virus

monoclonal antibodies

MEP HyperCelTM

transgenic plants

antibody purification

Protein A

Characterization of Transgenic Peanuts Expressing Oxalate Oxidase for Governmental Approval of Their Release for Control of Sclerotinia Blight

Chriscoe, Shanna Marie

28 July 2009

<i>Sclerotinia minor</i> Jagger is a fungal pathogen of cultivated peanut (<i>Arachis hypogaea</i> L.) that can cause crop losses in excess of 50%. Fungicides are not completely effective at controlling the disease and can cost up to $311 per hectare for three applications. The ability to produce oxalic acid is necessary for the pathogenicity of some <i>Sclerotinia</i> spp. With little to no naturally occurring resistance to Sclerotinia blight in <i>Arachis</i> spp., a biotechnological approach was used to confer resistance to the disease. Peanut plants were transformed with a gene from barley encoding oxalate oxidase, an enzyme that degrades oxalic acid. Transformed peanuts showed resistance to S. minor and increased yields under disease pressure compared to the parental lines. Before the resistant varieties can be marketed, they must be reviewed and approved by the governmental regulatory system. Responsibility for regulation of transgenic plants in the U.S. is shared among the U.S. Department of Agriculture (USDA) through the Animal and Plant Health Inspection Service (APHIS), the Food and Drug Administration (FDA), and the Environmental Protection Agency (EPA). These agencies require several different data sets including molecular characterization and field studies before each transformation event can be commercialized. This project was designed to characterize three different transformation events, N70, P39 and W171. Molecular characterization included determination of insertion number, copy number, intactness of the expression cassette and stable inheritance of the transgene. N70 was found to have two insertions and two copies while W171 had one insertion with one copy. The P39 event has two insertions and two or more copies. Each of the three events was stable over multiple generations. Phenotypic comparisons of each transgenic line to the parent cultivar were carried out in field studies. Characteristics such as oxalate oxidase expression, yield and quality, hay quality, disease occurrence, aflatoxin content and plant height were assessed. Transgenic peanuts showed few differences from the parent cultivar other than resistance to Sclerotinia blight and yield under disease pressure. Outcrossing studies were completed to determine the rate and distance of cross pollination. Outcrossing rates in N70, P39 and W171 were less than 2.5% and occurred up to 19 rows or 17.4 m from the nearest transgenic row. The molecular characterization and field performance of N70, P39 and W171 have been assembled into a document to petition APHIS for determination of non-regulated status. / Master of Science in Life Sciences

Sclerotinia blight

Sclerotinia minor

peanut

transgenic plants

governmental regulation

oxalate oxidase

Arachis hypogaea