Global ETD Search

21	The application of real-time PCR to investigate the effect of the arbuscular mycorrhizal fungus Glomus intraradices on the plant pathogen Fusarium solani f. sp. phaseoli / Filion, Martin January 2002 (has links) The effect of the arbuscular mycorrhizal symbiosis at reducing the incidence of root diseases has received considerable attention. However, information on the role of mycorrhizae in reducing disease incidence of Fusarium root rot of beans (Phaseolus vulgaris), caused by the root pathogen Fusarium solani f. sp. phaseoli, is scarce. A study was undertaken to investigate how the arbuscular mycorrhizal fungus (AMF) Glomus intraradices affects disease development and population number of F. solani f. sp. phaseoli in the mycorhizosphere of bean plants growing in an experimental microcosm unit. This newly designed unit facilitated the spatial monitoring and quantification of both the symbiont and pathogen in different ecological soil regions of the mycorrhizosphere using compartmentation based on a physical segregation of roots, colonized or not by AMF (rhizosphere), AMF mycelium alone (mycosphere), or none (bulk soil). To study the interaction between both organisms, the experimental set-up consisted of a randomized complete block design using bean seedlings pre-colonized or not for 28 days by G. intraradices and infected or not for 6 days with F. solani f. sp. phaseoli. Monitoring of population number of the symbiont and the pathogen in bean plants and in the different mycorrhizosphere soil compartments was achieved with quantitative real-time PCR using specific molecular probes for each fungus, and with cultivation-dependant or morphological based methods. The results of this study indicated that non-mycorrhizal bean plants infected with the pathogen had typical root rot symptoms while infected plants that were pre-colonized by G. intraradices remained free of disease. The population number of F. solani f. sp. phaseoli was significantly reduced in the root system and in each of the mycorrhizosphere soil compartments of mycorrhizal infected plants. The mycorrhizosphere population of G. intraradices was not significantly modified, although the p Beans -- Disease and pest resistance. Glomus intraradices. Vesicular-arbuscular mycorrhizas. Fusarium solani.
22	Production Of Anticancer Drug Taxol And Its Precursor Baccatin III By Fusarium Solani And Their Apoptotic Activity On Human Cancer Cell Lines Chakravarthi, B V S K 05 1900 (has links) (PDF) Taxol (generic name paclitaxel), a plant‐derived antineoplastic agent, was originally isolated from the bark of the Pacific yew, Taxus brevifolia. Obtaining taxol from this source requires destruction of trees. It has been used alone or in combination with other chemotherapeutic agents for the treatment of breast, ovarian as well as many other types of cancer, including non‐small cell lung carcinoma, prostate, head and neck cancer, and lymphoma, as well as AIDSrelated Kaposi’s sarcoma. The mode of action of taxol against a number of human cancer cells is by preventing the depolymerization of tubulin during cell division. This molecule increases microtubule stability in the cell and induces apoptosis. From yew trees, the yield of taxol is usually between 0.004 to 0.1% of the dry weight. The commercial isolation of 1 Kg of taxol requires about 6 to 7 tons of T. brevifolia bark obtained from 2000‐3000 well‐grown trees. The limited supply of the drug has prompted efforts to find alternative sources of taxol. Alternative methods for taxol production, such as chemical synthesis, tissue and cell cultures of the Taxus species are expensive and give low yields. A fermentation process involving any microorganism would be the most desirable means to lower the cost and increase availability. The first report on the isolation of taxol‐producing fungi from Taxus brevifolia appeared in 1993 (Stierle, et al., 1993). Several taxol‐producing fungi have been identified since, such as Taxomyces andreanae, Taxodium disticum, Tubercularia sp., Pestalotiopsis microspora, Alternaria sp., Fusarium maire and Periconia sp (Li, et al., 1996, Strobel, et al., 1996a, Strobel, et al., 1996b, Li, et al., 1998b, Ji, et al., 2006, Xu, et al., 2006). This thesis investigates the isolation of an endophytic fungus, isolated from the stem cuttings of Taxus celebica, which produces taxol and related taxanes. We observed morphological and cultural characteristics and analyzed the sequences of rDNA ITS from the strain. The isolated fungus grew on potato carrot agar (PCA) medium at 25 °C and the colonies were white to off‐white, floccose, with irregular margins. The reverse side of the culture was cream in color. The morphology was examined microscopically following staining with cotton blue in lactophenol. Cultures produced macroconidia on slender, 85 μm long phialides. The macroconidia were 25‐40 X 3.75 μm. Cultures also produced round or oval microconidia. Analysis of the ITS and D1/D2 26S rDNA sequence revealed 99 % identity with Fusarium solani voucher NJM 0271. Based on its morphological, cultural characteristics and 26S rDNA sequence, the fungus was identified as F. solani. This fungus is different from the previously reported endophytic taxol‐producing species of Fusarium. Taxol and baccatin III, produced by this fungus, were identified by chromatographic and spectroscopic comparison with standard compounds. The amount of taxol produced by F. solani in potato dextrose liquid medium is low (1.6 μg l‐1) (Chakravarthi, et al., 2008). We further investigated different growth media and various factors of cultivation to select the medium and conditions that maximize production of taxol and other taxanes by this fungus. F. solani was grown in five well‐defined culture media under stationary and shake conditions separately for various time intervals and the amounts of taxol, baccatin III and other taxanes produced were estimated by competitive immunoassay. The modified flask basal medium (MFBM) was shown to yield the highest production of taxol (128 μg l‐1) which is 80 times more than when grown in potato dextrose liquid medium, baccatin III (136 μg l‐1) and total taxanes (350 μg l‐1) under shake conditions. From our results the highest taxol production of F. solani was achieved when cultured in MFBM. The production in MFBM was 80 times higher than that cultured in the potato dextrose liquid medium. In conclusion, it was shown that the culture medium plays a major role in taxol and other taxanes production and fungal growth. MFBM is the best medium, among the media studied, to produce taxol and other taxanes. The higher concentrations of NH4NO3, MgSO4, KH2PO4 and FeCl3 in the FBM medium seem important for production of taxol and other taxanes. These results can be considered as starting‐point for the research directed to improve taxol and baccatin III production by F. solani via different approaches including fermentations, strain improvement and genetic engineering techniques. Finally, in order to get more insights into the mode of action of this fungal taxol and baccatin III (for the first time), their apoptotic activity on different cancer cell lines was determined. We elucidated the biochemical pathways leading to apoptotic cell death after fungal taxol‐ and baccatin III‐ treatment in different cancer cell lines. Experiments are done on various cancer cell lines namely JR4 Jurkat (T‐cell leukemia), J16 Bcl‐2 Jurkat T cells, HepG2 (hepatoma), caspase‐8‐deficient Jurkat T cells, HeLa (human cervical carcinoma), Ovcar3 (human ovarian carcinoma) and T47D (human breast carcinoma) cells. We were able to demonstrate that both fungal taxol and baccatin III can induce apoptosis in all the cell lines tested, by flow cytometric analysis. Hallmarks of apoptosis following the signaling pathway to far more upstream‐located events were investigated using biochemical and cell biological methods. It has shown that during fungal taxol‐ and baccatin III‐induced apoptosis, DNA is degraded resulting in a increased number of hypodiploid cells reaching up to 65‐70% after 48 h. Disruption of mitochondrial membrane potential was examined by flow cytometric analysis using mitochondrial membrane potential sensitive dye JC‐1 and JR4‐Jurkat cells were shown to undergo significant loss of mitochondrial membrane potential loss of mitochondrial membrane potential reaching up to 70% in 6 nM fungal taxol and 65 % in 3.5 μM baccatin III after 36 h. These results were similar to those observed with standard taxol and baccatin III. We further investigated the role of caspases in fungal taxol‐ and baccatin III‐induced apoptosis, caspase‐8‐deficient Jurkat cells, Bcl‐2‐over‐expressed J16‐Jurkat cells and caspase inhibitors were used. Results derived from caspase‐8‐deficient Jurkat cells show that caspase‐8 is not involved in fungal taxol‐ and baccatin IIIinduced apoptosis of Jurkat cells. Using the pan‐caspase inhibitor (Z‐VAD‐FMK), caspase‐9 inhibitor (Z‐LEHD‐FMK), caspase‐3‐inhibitor (Z‐DEVD‐FMK), caspase‐2‐ inhibitor (Z‐VDVAD‐FMK) and caspase 10‐inhibitor (Z‐AEVD‐FMK), it was shown that caspase‐10 is involved in fungal taxol‐ and baccatin III‐ induced apoptosis in JR4‐Jurkat cells. It was also shown that inhibitors of caspases‐9, ‐2 or ‐3 partially inhibited fungal taxol‐ and baccatin III‐ induced apoptosis, whereas the caspase‐ 10 inhibitor totally abrogated this process. With the use of a fluorescence microscope, several morphological features characteristic of apoptosis such as condensed chromatin and apoptotic bodies were identified in fungal taxol‐ and baccatin III‐treated JR4‐Jurkat and HeLa cells. DNA fragmentations were shown by agarose gel electrophoresis method. Our work showed that treatment of JR4‐ Jurkat and HepG2 cells with fungal taxol and baccatin III induces apoptosis as shown by DNA ladder formation. Herein it was demonstrated that fungal taxol and baccatin III have a similar mechanism of action, but the efficacy of fungal taxol to induce apoptosis is higher. In summary, fungal baccatin III is found to be effective in inducing apoptosis similar to taxol but at higher concentration and both fungal taxol and baccatin III induce apoptosis via caspase‐10 and mitochondrial pathway in Jurkat cells. In conclusion, the present study describes isolation of a taxol‐producing endophyte F. solani IISc.CJB‐1. The growth requirements of this fungus for production of taxol, baccatin III and other taxanes were studied. The apoptotic activity of taxol and baccatin III (for the first time) was observed. In addition, our results show that the culture medium plays a major role in taxol and other taxanes production and fungal growth. Among the media studied, modified flask basal medium (MFBM) is the best to produce taxol and other taxanes. It is evident from this data that this fungal strain can be promising candidate for large‐scale production of taxol and related taxanes. Fusarium Solani Anticancer Drugs Cancer - Therapy Chemotherapy Taxol - Synthesis Taxanes Apoptosis Paclitaxel Baccatin Taxus celebica Pharmacology
23	The application of real-time PCR to investigate the effect of the arbuscular mycorrhizal fungus Glomus intraradices on the plant pathogen Fusarium solani f. sp. phaseoli / Filion, Martin January 2002 (has links) No description available. Fusarium solani. Glomus intraradices. Vesicular-arbuscular mycorrhizas. Beans -- Disease and pest resistance.
24	Effect of <i>Aloe striata</i> Inner Leaf Gel on Early Hyphal Development and Adhesion in <i>Paecilomyces variotii</i>, <i>Fusarium oxysporum</i>, and <i>Fusarium solani</i> Wada, Gloria Achibi 29 March 2016 (has links) No description available. Biology Microbiology Adhesion Paecilomyces variotii Fusarium oxysporum Fusarium solani Aloe striata
25	Identification et détection d'une nouvelle espèce de Fusarium pathogène sur la tomate de serre en Amérique du Nord Moine, Lauriane 19 April 2018 (has links) Récemment, un nouvel agent pathogène a causé d’importants dommages sur la tomate de serre dans un complexe au centre du Québec et au nord des États-Unis. À partir d’échantillons de plants infectés, des colonies produisant des macroconidies typiques de Fusarium spp. ont systématiquement été isolées. Le séquençage des régions ITS et tef de ces isolats, suivi de tests de pathogénicité, ont permis d’identifier Fusarium striatum comme l’agent pathogène. Il s’agit du premier rapport de cet agent pathogène au Canada. Suite à son identification, un test de dépistage moléculaire a été mis au point afin de détecter l’agent pathogène directement à partir des tissus végétaux. Les amorces développées ont été suffisamment spécifiques et sensibles pour détecter l’agent pathogène avant même l’apparition des symptômes. Nos résultats semblent indiquer que l’inoculum de F. striatum aurait été introduit dans les deux complexes de serre par les transplants provenant de leur fournisseur commun. S 405 UL 2013 Fusarium solani -- Identification
26	Populações de fungos fitopatogênicos e concentrações de nutrientes no solo em pomares de fruteiras temperadas adubados com Dejeto suíno compostado / Pathogenic fungi populations and nutrient concentrations in soil in orchards of temperate fruit trees fertilized with swine manure composted Costa Junior, Avanor Cidral da 31 July 2014 (has links) Made available in DSpace on 2016-12-08T16:44:49Z (GMT). No. of bitstreams: 1 PGPV14MA158.pdf: 622907 bytes, checksum: 4bef911008ae5cffa26706180f710db4 (MD5) Previous issue date: 2014-07-31 / Coordenação de Aperfeiçoamento de Pessoal de Nível Superior / The addition and incorporation of organic matter to the soil, besides favoring crops by improving soil physical, can increase nutrients and add specific biochemicals capable of renewing the native microflora and microfauna. These compounds may, depending on the organic material to act as a suppressant effect and biocontrol. The aim of this study was to evaluate the effect of swine manure compost (DSC) in an orchard of apple, pear and grape vines on the population dynamics of Verticillium dahliae, Fusarium solani, Fusarium oxysporum, Fusarium verticillioides and Trichoderma sp. Soil samples for quantification of fungal colonies and nutrient analysis were collected at a depth of 0-10 cm soil of the orchard with apple, pear and grape vines. The population of pathogenic soil fungi and Trichoderma sp. were obtained by dilution and plating of 10 g of soil samples from soil orchard who received two doses of DSC (50 to 100%) compost and two (50 and 100%), using two culture media (BDA potato-dextrose-agar) and Sabouraud-ágar-chloramphenicol. The application of different doses of DSC and chemical fertilizer began in December 2012, repeated at intervals of 60 days until the 2014 harvest analysis of macronutrients (nitrogen, phosphorus, potassium, calcium and magnesium) and micronutrients (iron, copper, zinc and Manganese) DSC and chemical fertilizer were run using Mehlich-1, spectrophotometry, acid-base titration and Kjeldahl method, all described by Tedesco et al. (1995). Results in the concentration of nutrients was related to the population of Verticillium dahliae, Fusarium solani, Fusarium oxysporum, Fusarium verticillioides and Trichoderma sp. The experimental design was completely randomized, factorial 2 x 5, repeated in time (months). The data were analyzed using the MIXED procedure of SAS (SAS Inst. Inc., Cary, NC, v.9.2) and mean comparisons using Tukey least significant difference p ≤ 0.05. In the apple orchard, Fusarium oxysporum and Fusarium solani showed higher populations in Q100 treatments (0-110 x 103 CFU / g of soil) and Q50 (0-70 x 103 CFU/g of soil) respectively. There were differences in the population periods. Phosphorus, Potassium and Sodium showed significant differences among the treatments tested. In the orchard of pear trees the largest population of Fusarium solani was the S100 treatment (0-50 x 103 CFU/ g of soil). Treatments Q50 and Q100 had higher populations of Verticillium dahliae, Fusarium oxysporum and Fusarium verticillioides in different periods. Concentrations of Nitrogen and Potassium differ between treatments tested. In vineyards the largest populations of Fusarium solani and Fusarium oxysporum were found in December-2012 periods (0-70 x 103 CFU / g of soil) and August 2013 (0-60 x 103 CFU / g of soil) respectively. Concentrations of potassium, phosphorus and sodium were higher in treatment S50 and S100. The orchard of apple, pear and grape vines have different response to chemical and organic fertilization. The intensity of response to fertilization has little influence population dynamics of plant pathogens in soil and Trichoderma / A adição e incorporação de matéria orgânica ao solo, além de favorecer as culturas pela melhoria física do solo, podem potencializar nutrientes e adicionar compostos bioquímicos específicos capazes de renovar a microfauna e microflora nativas. Estes compostos podem, dependendo do material orgânico, agir como efeito supressor e como biocontrole. O objetivo deste trabalho foi avaliar o efeito da aplicação de dejeto suíno compostado (DSC) em pomar de macieiras, pereiras e videiras, sobre a dinâmica populacional de Verticillium dahliae, Fusarium solani, Fusarium oxysporum, Fusarium verticillioides e Trichoderma sp. Amostras de solo para quantificação de colônias fúngicas e análise de nutrientes foram retiradas na profundidade 0-10 cm de solo do pomar de macieiras, pereiras e videiras. A população de fungos fitopatogênicos de solo e Trichoderma sp. foram obtidas pela diluição e plaqueamento de 10 g de amostras de solo provenientes do solo do pomar que receberam duas doses de DSC (50 e 100%) e duas de adubo químico (50 e 100%), utilizando dois meios de cultura, BDA (batata-dextrose-agar) e Sabouraud ágar-cloranfenicol. A aplicação das diferentes doses de DSC e adubo químico tiveram início em dezembro-2012, repetidas em intervalos de 60 dias até a safra 2014. A análise dos macronutrientes (nitrogênio, fósforo, potássio, cálcio e magnésio) e micronutrientes (ferro,cobre,zinco e Manganês) do DSC e da adubação química foram realizados pelos métodos de Mehlich -1, espectrofotometria, titulação ácido-base e método Kjeldahl, todas descritas por Tedesco et al. (1995). Resultados da concentração de nutrientes foi relacionado à população de Verticillium dahliae, Fusarium solani, Fusarium oxysporum, Fusarium verticillioides e Trichoderma sp. O delineamento experimental foi inteiramente casualisado, em arranjo fatorial 2 x 5, repetidos no tempo (meses). Os dados foram analisados pelo procedimento MIXED do SAS (SAS Inst. Inc., Cary, NC, v.9.2) e as comparações de médias usando a diferença mínima significativa de Tukey p ≤ 0,05. No pomar de macieiras, Fusarium oxysporum e Fusarium solani apresentaram maiores populações nos tratamentos Q100 (0-110 x 103 UFC/g de solo) e Q50 (0-70 x 103 UFC/g de solo) respectivamente. Houve diferenças da população nos períodos avaliados. Fósforo, Potássio e Sódio apresentaram diferenças significativas entre os tratamentos testados. No pomar de pereiras a maior população de Fusarium solani foi ao tratamento S100 (0-50 x 103 UFC/g de solo). Os tratamentos Q50 e Q100 apresentaram maiores populações de Verticillium dahliae, Fusarium oxysporum e Fusarium verticillioides em diferentes períodos de avaliação. Concentrações de Potássio e Nitrogênio apresentaram diferenças nos tratamentos testados. Na cultura da videira as maiores populações de Fusarium solani e Fusarium oxysporum foram encontradas nos períodos dezembro-2012 (0-70 x 103 UFC/g de solo) e agosto-2013 (0-60 x 103 UFC/g de solo) respectivamente. Concentrações de Potássio, Fósforo e Sódio foram superiores nos tratamento S50 e S100. O pomar de macieiras, pereiras e videiras apresentam diferentes resposta a adubação química e orgânica. A intensidade de resposta da adubação pouco influencia a flutuação da população de fitopatógenos de solo e Trichoderma Verticillium dahliae Fusarium solani Fusarium oxysporum Fusarium verticillioides Trichoderma sp. dejeto suíno compostado flutuação populacional Verticillium dahliae Fusarium solani Fusarium oxysporum Fusarium verticillioides Trichoderma sp swine manure composted population fluctuation CNPQ::CIENCIAS AGRARIAS::AGRONOMIA
27	Análise de variabilidade genética e obtenção de protoplastos do fungo Fusarium solani f. sp. glycines, agente causal da síndrome da morte súbita em soja (Glycine max L. Merrill) / Genetic variability and protoplasts isolation of Fusarium solani f. sp. glycines, the causative agent of sudden death syndrome in soybean (Glycine max L. Merrill) Aleixo, Luciana Aguilar 26 June 2003 (has links) Submitted by Marco Antônio de Ramos Chagas (mchagas@ufv.br) on 2017-06-01T18:40:48Z No. of bitstreams: 1 texto completo.pdf: 2130474 bytes, checksum: b9156f2bfd2a4a0f4c702f5e05f2d6c3 (MD5) / Made available in DSpace on 2017-06-01T18:40:48Z (GMT). No. of bitstreams: 1 texto completo.pdf: 2130474 bytes, checksum: b9156f2bfd2a4a0f4c702f5e05f2d6c3 (MD5) Previous issue date: 2003-06-26 / Conselho Nacional de Desenvolvimento Científico e Tecnológico / Fusarium solani f. sp. glycines, agente causal da síndrome da morte súbita em soja, é um importante patógeno no Brasil e em outras partes do mundo. Foram obtidos 15 isolados de F. solani f. sp. glycines a partir de 57 fragmentos de raíz de soja coletados em diferentes localidades no Brasil. A diversidade genética destes 15 isolados e de outros 4 isolados cedidos pelo Departamento de Fitotecnia da Universidade Federal de Viçosa, foi avaliada por RAPD. As amplificações com 15 oligonucleotídeos resultaram em 175 fragmentos polimórficos e 5 monomórficos. As distâncias genéticas entre os isolados variaram de 12,2 a 85%, revelando alta variabilidade genética. Não houve agrupamento dos isolados de acordo com seu local de coleta. Esta alta variabilidade genética provavelmente se deve à presença de transposons e de ciclo parassexual do patógeno. Protoplastos de Fusarium solani f. sp. glycines foram obtidos por digestão enzimática do micélio, na presença de MgSO 4 1,2 M como estabilizador osmótico. Foram liberados 2,4 X 10 7 protoplastos/mL após 4 horas de digestão do micélio a 28°C e 80 rpm. A concentração ideal de enzima lítica para a protoplastização foi de 15 mg/mL. A maior taxa de regeneração dos protoplastos foi de 5,5% em meio BDA estabilizado com sacarose 1,0 M. / Fusarium solani f. sp. glycines, the causative agent of sudden death syndrome in soybean, is an important pathogen in Brazil and in other parts of the world. Fifteen F. solani f. sp. glycines isolates were obtained out of 57 root fragments collected in different growing regions in Brazil. The genetic diversity of these isolates and that of four isolates obtained from the Department of Plant Sciences of the Federal University of Viçosa were analyzed by RAPD. Amplification with 15 primers resulted in 175 polymorphic and 5 monomorphic DNA fragments. The genetic distances among the isolates ranged from 12.2 to 85%. No grouping was obtained based on geographic localization, certainly because there were not enough differentiation. This high genetic variability is probably due to the activity of transposons and the presence of the parassexual reproduction. Fusarium solani f. sp. glycines protoplasts were obtained by enzymatic digestion of micelium, using 1,2 M MgSO 4 as osmotic stabilizer. Aproximately 2.4 X 10 7 protoplasts/mL were obtained after 4 hours of micelium digestion at 28°C e 80 rpm. The optimum enzyme concentration was 15 mg/mL. The highest protoplast regeneration rate was 5.5% in BDA stabilized with 1,0 M sucrose. / Dissertação importada do Alexandria Fusarium solani f. sp. glycines Síndrome da morte súbita em soja Obtenção de protoplastos Ciências Agrárias
28	Produkce a charakterizace extracelulárních hydroláz z vybraných druhů plísní / Production and characteritzation of extracellular hydrolases from selected moulds Skoumalová, Petra January 2011 (has links) This diploma thesis is focused on study of potential production of extracellular hydrolytic enzymes. The theoretical part deals with characterization of selected hydrolytic enzymes, their catalytic properties, the possibility of extracellular hydrolase production by fungi and their applications. In experimental part production strains Aureobasidium pullulans, Fusarium solani and Phanerochaete chrysosporium were used. Productions of cellulase, amylase, xylanase, lipase, protease and lignin-degraded enzymes (laccase, manganese- dependent peroxidase, lignin peroxidase) were observed. Cultivations were carried out in submersed mode in mineral medium supplemented by waste co-substrates such as wheat bran, corn bran, rice bran and oat bran, sawdust, rice, apple fiber, egg pasta and egg-free pasta. Production of enzymes depended on the substrate type and time of cultivation. The highest cellulase, xylanase and amylase activities were measured in the first period of cultivation (3 to 7 day). Lignin-degraded enzymes and proteases were produced at the end of cultivation (7 to 10 days). Lipolytic activity was detected only in A. pullulans, where the activity increased with time of cultivation. The highest value was determined during cultivation on wheat bran (3.6 nmol/ml.min). The highest xylanase and celulase activity (170.3 nmol/ml.min, 248.0 nmol/ml.min) were determined during cultivation of F. solani on corn bran. The highest amylase activity (111.8 nmol/ml.min) was reported in P. chrysosporium during the cultivation on rice. The highest protease activity (68.0 nmol/ml.min) was determined in F. solani grown on wheat bran. The best producer of laccase was A. pullulans, the highest production was recorded for egg-free pasta (27.0 nmol/ml.min). The maximum lignin peroxidase activity (12.5 nmol/ml.min) was measured during the cultivation of F. solani on egg pasta, while the highest yield of Mn-dependent peroxidase (7.7 nmol/ml.min) was achieved during the cultivation of A. pullulans on wheat bran. Lignin-degraded enzymes behaved as inductive, while the other enzymes were produced in mineral medium too. Activity of cellulase in the mineral medium was in A. pullulans strain higher than in media with waste substrates. Enzymes produced into A. pullulans medium were purified by ultrafiltration, ion exchange chromatography and gel filtration.
29	Rezistence odrůd hrachu setého k houbovým patogenům Slováková, Michaela January 2018 (has links) The diploma thesis concerns observing the health conditions of pea plants. The experiments were established in 2016–2017 in cooperation with AGRITEC, research, breeding and services, s.r.o. company in Šumperk. There were 9 varieties and 3 lines selected for the experimentations. The observation for each experiment was divided into two timing terms. The resistance to pea powdery mildew caused by pathogen Eryshipe pisi, was observed in greenhouse conditions. The highest level of resistance occurred line 1109/13 and variety FRANKLIN. The lowest level of resistance had variety ARVIKA. However this variety also occured to have the highest level of resistance in laboratory tests to resistance to Fusarium solani and Fusarium oxysporum. The pathogens causing the complex of root rot and black stem deseases were observed in conditions of infectious field. Variety ATLAS was infected the least.
30	Estratégias de seleção de genótipos de soja para resistência à podridão vermelha das raízes / Selection strategies of soybean genotypes resistant to sudden death syndrome Bernardi, Walter Fernando 01 September 2008 (has links) Nas últimas décadas, a podridão vermelha das raízes da soja (PVR), causada pelo Fusarium solani f.sp. glycines (FSG), tornou-se uma doença séria nas regiões brasileiras onde já foi constatada, sendo a utilização de cultivares resistentes um componente fundamental de um sistema integrado de controle. Este trabalho teve por objetivo pesquisar estratégias de seleção de genótipos resistentes a PVR. Várias metodologias foram implementadas: avanço de progênies até a geração F7:2 e seleção em campo infestado, de progênies selecionadas em F2. Avaliou-se o cruzamento IAC 4 x Conquista em casa de vegetação (geração F3:2) e em campo infestado (gerações F3:2, F4:2 e F5:2), através de estudo de estabilidade e adaptabilidade das progênies. As metodologias de infecção em vasos de barro e bandejas de isopor em casa de vegetação foram comparadas para melhorar a eficiência de seleção; também foi feita análise de repetibilidade dos sintomas foliares da PVR, para otimização do número de avaliações necessárias para classificar o genótipo de soja quanto à reação ao FSG. Cultivares brasileiras de soja foram avaliadas em campo infestado. Em campo, as plantas foram avaliadas no estádio R5-6, com notas variando de 1 (ausência de sintomas) a 5 (100% da raiz principal com sintomas). Em casa de vegetação, as plantas foram avaliadas aos 35 dias pós-semeadura para sintomas radiculares e da parte aérea. Houve eficiência da seleção para resistência a PVR tanto em F2 (sintomas foliares em casa de vegetação) quanto em F7:2 (sintomas radiculares em campo naturalmente infestado). A seleção praticada nas gerações intermediárias também foi eficiente para aumentar a produtividade de grãos das progênies. Para o cruzamento IAC 4 x Conquista nas gerações F3:2, F4:2 e F5:2 em campo naturalmente infestado e na F3:2 em casa de vegetação, a metodologia de Annicchiarico possibilitou a seleção de genótipos com maior estabilidade e adaptabilidade para os diferentes ambientes; com o estudo genético destas gerações, demonstrou que há efeitos gênicos aditivos e dominantes no controle genético da PVR. Além disso, constatou-se que os genes responsáveis pela resistência estão dispersos nos genitores, provavelmente agrupados em blocos gênicos. A presença de dominância indica que a seleção deve ser postergada para gerações com maior homozigose (linhagem pura); esta idéia foi reforçada pela baixa herdabilidade ao nível de plantas. O uso de bandejas de isopor foi significativamente mais eficiente do que vasos de barro para inoculação de FSG em casa de vegetação. Pela análise de repetibilidade, detectou-se que quatro avaliações foram suficientes para discriminar se o genótipo era realmente suscetível ao FSG. A correlação da geração F3:2 (IAC 4 x Conquista) entre campo infestado e casa de vegetação foi praticamente nula; no entanto, 54% das progênies selecionadas em campo também foram selecionadas em casa de vegetação. A seleção de genótipos superiores para resistência ao FSG não é tarefa fácil, mas pode ser aprimorada pelo uso conjugado de metodologias suplementares que aumentem a eficiência de seleção. / During the last decades, soybean sudden death syndrome (SDS), caused by Fusarium solani f.sp. glycines (FSG), has become a serious disease in the regions where it was encountered. The use of resistant soybean cultivars has been an important component of an integrated management system. The aim of this work was to research selection strategies of SDS-resistant genotypes. A number of methodologies were used: self pollination up to generation F7:2 and progeny selection in infested field of selected F2. The crossing IAC 4 x Conquista was studied in greenhouse (generation F3:2) and in a naturally infested field (generations F3:2, F4:2 and F5:2), where the progeny stability and adaptability study was carried out. The methodologies of infection in clay pots and polystyrene trays in greenhouse were compared to improve selection efficiency. An analysis of the repeatability of foliar SDS symptoms was also performed in order to optimize the number of evaluations needed to classify a soybean genotypes reaction to FSG. Brazilian soybean cultivars were evaluated in a naturally infested field, where plants were evaluated at stage R5-6 with scores varying from 1 (absence of symptoms) to 5 (main root 100% symptoms). In the greenhouse, the plants were evaluated 35 days after sowing for root symptoms, while the leaf symptoms was only evaluated after the appearance of symptoms. The selection done in F2 (leaf symptoms in greenhouse) as well as F7:2 (root symptoms in infested field) for FSG were efficient. The selections performed in intermediary generations were efficient in increasing the grain yield of the progeny. Studies of the F3:2, F4:2 and F5:2 generations of the IAC 4 x Conquista cross in an infested field and F3:2 in greenhouse, enabled through Annicchiaricos methodology, the selection of genotypes with greater stability and adaptability to different environments. The genetic study of these generations demonstrated there are additive and dominant genetic effects on the genetic control of SDS. Moreover, it was noted that the genes responsible for resistance are dispersed on the genitors, probably grouped into genic blocks. The presence of dominance indicates that the selection should be passed onto generations with greater homozygosity. There is also a clear indication that breeders should work with progeny lines in order to assist selection due to the low inheritability at the individual plant level. For the experiments with different FSG inoculation methodologies (clay pots and polystyrene trays) in greenhouse the use of trays was significantly more efficient; by studying the repeatability analysis, it was found that four evaluations is enough to discriminate if the genotype is really susceptible to FSG. The correlation of the F3:2 generation (IAC 4 x Conquista) between infested field and greenhouse was practically null; however, 54% of the progeny selected in the field were selected in greenhouse. As observed, the selection of superior genotypes for FSG resistance is not an easy task, but may be improved by means of new methodologies and the conjugated use of methodologies which improve selection efficiency. Fusariose vegetal Fusarium solani f.sp. glycines Glycine max Grãos - Produtividade Hereditariedade Inheritance of genetic resistance Podridão (Doença de planta) Resistência genética vegetal Seed yield. Soja. Sudden death syndrome

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