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251	Uso de reguladores de crescimento e controle biológico de fungos no feijoeiro cultivado em sucessão à dife-rentes culturas de cobertura / Use of growth regulators and biological control of fungi in the common bean cultivated in succession to different cover crops BERNARDES, Tatiely Gomes 25 February 2008 (has links) Made available in DSpace on 2014-07-29T16:24:14Z (GMT). No. of bitstreams: 1 DISSERTACAO TATIELY GOMES BERNARDES 2008.pdf: 436182 bytes, checksum: ed86a8aa78f5feb99af31d615243e746 (MD5) Previous issue date: 2008-02-25 / In order to increase the productivity of the common bean crop several technologies are offered, but there is lack of studies to verify their efficiency. The objective of this work was to evaluate the effect of growth regulator and the biological control of fungi of the soil through Trichoderma sp., seeking larger productivity of the commom bean plant irrigated in succession to different cover crops. The experiments were conducted in Fazenda Capivara - Embrapa Arroz e Feijão, in the municipality of Santo Antônio de Goiás, GO, in a Dystrophic Red Latosol. The experimental design was a randomized complete block on split-plot, with four replications. The plots of the two experiments consisted of cultures used as soil cover, as the leguminous: pigeon pea (Cajanus cajan L. Millisp), Stylosanthes guianensis cv. Campo Grande, and Crotalária spectabilis Roth., and the grasses: millet (Pennisetum glaucum L. R. Br.), Panicum maximum cv. Mombaça, Brachiaria brizantha cv. Marandu, B. brizantha associated with corn (Zea mays L.) and sorghum (Sorghum bicolor L. Moench). To the 84 days after the cut of the cover crops common bean cultivar BRS Valente was sown under central pivot. Experiment 1: the subplot treatments were: a) control; b) 500 ml of growth regulator (RC - commercial product Stimulate) in 100 kg of seeds; c) 1250 ml of biological fungicide (FB - commercial product Trichodermil) in 100 kg of seeds; and, d) 500 ml of RC plus 1250 ml FB in 100 kg of seeds. They were evaluated severity of root rot, incidence of fusarium wilt, grain yield, mass of 100 grains, number of beans for plant, number of grains for bean and initial and final stand of the commom bean. Experiment 2: the subplots consisted of the following treatments: a) control; b) 500 ml of growth regulator (RC - commercial product Stimulate) in 100 kg of seeds; c) 250 ml of RC for hectare in the V4 development stage, foliar treatment; and, d) 500 ml RC in 100 kg of seeds and 250 ml of RC for hectare via foliar, in the V4 development stage. They were evaluated the grain yield, mass of 100 grains, number of beans for plant, number of grains for bean and initial and final stand of the commom bean. The obtained data of the studied variables were submitted to the variance analyses being applied the F test, and when there were differences among the averages, these were compared by the Tukey test at 5% of probability. Experiment 1: The treatments with Trichoderma sp. and growth regulators applied via seeds did not showed significant effect in the analyzed variables. The sorghum straw favored the increase of the severity of the root rot and of the fusarium wilt in the common bean crop, causing a lower grain yield. The highest grain yield was obtained in the millet straw. Experiment 2: The treatments with growth regulator applied via seeds and foliar did not significantly influenced the common bean grain yield. The predecessor cover crops influenced the common bean grain yield, and the millet was that provided the largest common bean grain yield. / Visando aumentar a produtividade do feijoeiro várias tecnologias são oferecidas, mas faltam estudos para verificar a eficiência destas. O objetivo deste trabalho foi avaliar o efeito de regulador de crescimento e o controle biológico de fungos do solo por meio de Trichoderma sp., visando maior produtividade do feijoeiro irrigado em sucessão à diferentes culturas de cobertura. Os experimentos foram conduzidos na Fazenda Capivara Embrapa Arroz e Feijão, no município de Santo Antônio de Goiás, GO, em Latossolo Vermelho distrófico. O delineamento experimental foi em parcelas subdivididas, em blocos completos ao acaso com quatro repetições. Na parcela dos dois experimentos constaram às culturas utilizadas como coberturas do solo, as leguminosas: guandu, estilosante e crotalária, e as gramíneas: milheto, mombaça, braquiária, braquiária consorciada com milho e sorgo. Aos 84 dias após o corte das culturas de cobertura foi realizado a semeadura do feijoeiro, cultivar BRS Valente, sob pivô central. Experimento 1: nas subparcelas os tratamentos foram: a) testemunha; b) 500 ml de regulador crescimento (RC produto comercial Stimulate) em 100 kg de sementes; c) 1250 ml de fungicida biológico (FB produto comercial Trichodermil) em 100 kg de sementes; e, d) 500 ml de RC com mais 1250 ml FB em 100 kg de sementes. Foram avaliadas a severidade de podridão radicular, incidência de murcha-de-fusário, rendimento de grãos, massa de 100 grãos, número de vagens por planta, número de grãos por vagem e estande inicial e final do feijoeiro. Experimento 2: nas subparcelas constaram os seguintes tratamentos: a) testemunha; b) 500 ml de regulador de crescimento (RC - produto comercial Stimulate) em 100 kg de sementes; c) 250 ml de RC por hectare no estágio de desenvolvimento V4, tratamento foliar; e, d) 500 ml RC em 100 kg de sementes e 250 ml de RC por hectare via foliar, no estágio de desenvolvimento V4. Foram avaliados o rendimento de grãos, massa de 100 grãos, número de vagens por planta, número de grãos por vagem e estande inicial e final.do feijoeiro. Os dados obtidos das variáveis estudadas foram submetidos às análises de variância aplicando-se o teste de F, e quando houve diferença entre as médias, estas foram comparadas pelo teste de Tukey a 5% de probabilidade. Experimento 1: Os tratamentos com Trichoderma sp. e reguladores de crescimento aplicados via sementes não apresentaram efeito significativo em relação as variáveis analisadas. A palhada de sorgo favoreceu o aumento da severidade das podridões radiculares e da murcha-de-fusário no feijoeiro, causando um menor rendimento do feijoeiro. O maior rendimento do feijoeiro foi obtido na palhada de milheto. Experimento 2: Os tratamentos com reguladores de crescimento aplicado via sementes e foliar não influenciaram significativamente no rendimento do feijoeiro. As plantas de cobertura antecessoras influenciaram no rendimento do feijoeiro, sendo que o milheto foi a cobertura que proporcionou maior rendimento do feijoeiro. hormônios vegetais Trichoderma sp. Phaseolus vulgaris L. sistema plantio direto Cerrado vegetable hormones Trichoderma sp. Phaseolus vulgaris L. no-tillage system Cerrado
252	Nouvelles enzymes fongiques pour l'amélioration de la dégradation de la biomasse lignocellulosique : étude des "Lytic Polysaccharide Monooxygenases" (LPMOs) / New fungal enzymes for the improvement of lignocellulosic biomass degradation : study of the "Lytic Polysaccharide Monooxygenases" (LPMOs) Bennati-Granier, Chloe 02 February 2016 (has links) Dans le contexte actuel, il devient nécessaire de rendre les alternatives au pétrole, tel que le bioéthanol 2G, disponibles à grande échelle. Cependant, l’étape d’hydrolyse par les enzymes de Trichoderma reesei reste un verrou à un procédé économiquement stable et rentable. Ces travaux de thèse, s'intègrent dans le cadre du projet Futurol et ont pour objectifs d'identifier et de caractériser de nouvelles enzymes fongiques pour améliorer l'hydrolyse de la biomasse lignocellulosique. A partir des données protéomiques disponibles pour Podospora anserina et Fusarium verticillioides, une douzaine d'enzymes candidates ont été identifiées dans leurs sécrétomes. Ce travail de thèse s'est plus particulièrement focalisé sur les AA9s « Lytic Polysaccharide Monooxygenases » (LPMOs) de P. anserina. Parmi les LPMOs étudiées, PaLPMO9A, PaLPMO9E et PaLPMO9H, qui possèdent un CBM1, sont les plus actives sur la cellulose. La détermination de la régiosélectivité d'action a mis en évidence que PaLPMO9A et PaLPMO9H clivent la cellulose en position C1 et C4 alors que la PaLPMO9E génère uniquement des produits oxydés en C1. La PaLPMO9H est la plus versatile puisqu’elle est active sur les cello-oligosaccharides solubles et sur les polysaccharides hémicellulosiques liés en β-(1,4) (i.e., xyloglucane, glucomannane). La supplémentation du cocktail de T. reesei avec PaLPMO9E ou PaLPMO9H a permis de doubler les rendements d'hydrolyse du miscanthus prétraité. Les travaux réalisés au cours de cette thèse ont permis de démontrer l'importance de ces enzymes oxydatives dans les phénomènes de déconstruction de la lignocellulose chez les champignons filamenteux. / In the current context, it becomes essential to make alternative to oil, such as the 2G bioethanol, available at large scale. However, the hydrolysis step by Trichoderma reesei enzymes remains the major bottleneck for an economically sustainable process. The present work is part of the Futurol project, and aims at identifying and characterizing new fungal enzymes to improve the hydrolysis of lignocellulosic biomass. From the proteomic data available for Podospora anserina and Fusarium verticillioides, a dozen of interesting enzymes were identified in their secretomes. This work focuses, mainly, on the AA9s « Lytic Polysaccharide Monooxygenases » (LPMOs) from P. anserina. Among all the LPMOs studied, PaLPMO9A, PaLPMO9E and PaLPMO9H that harbored a CBM1 were the most active on cellulose. Investigation of their regioselective mode of action revealed that PaLPMO9A and PaLPMO9H oxidatively cleaved at both C1 and C4 positions while PaLPMO9E released only C1-oxidized products. PaLPMO9H that was the most versatile in terms of substrate specificity as it also displayed activity on cello-oligosaccharides and β-(1,4)-linked hemicellulose polysaccharides (e.g., xyloglucan, glucomannan). The hydrolysis yield of the pretreated miscanthus was significantly improved up to 2 fold, when the PaLPMO9E, or PaLPMO9H were supplemented to the T. reesei cocktail. This work demonstrated the importance of these oxidative enzymes for lignocellulose deconstruction by fungi. These biocatalysts open new prospects to improve the enzymatic conversion of plant biomass for 2G bioethanol production. Bioéthanol Aa9 lpmo Cellobiose déshydrogénase Cello-Oligosaccharides oxydés Clivage oxydatif Lignocellulose Podospora anserina Miscanthus Hydrolyse Trichoderma reesei Bioethanol Aa9 lpmo Cellobiose dehydrogenase Oxidized cello-Oligosaccharides Oxidative cleavage Lignocellulose Podospora anserina Miscanthus Hydrolysis Trichoderma reesei 579
253	Solid state fermentation of soybean hulls for cellulolytic enzymes production: physicochemical characteristics, and bioreactor design and modeling Brijwani, Khushal January 1900 (has links) Doctor of Philosophy / Department of Grain Science and Industry / Praveen V. Vadlani / The purpose of this study was to investigate micro- and macro-scale aspects of solid state fermentation (SSF) for production of cellulolytic enzymes using fungal cultures. Included in the objectives were investigation of effect of physicochemical characteristics of substrate on enzymes production at micro-scale, and design, fabrication and analysis of solid-state bioreactor at macro-scale. In the initial studies response surface optimization of SSF of soybeans hulls using mixed culture of Trichoderma reesei and Aspergillus oryzae was carried out to standardize the process. Optimum temperature, moisture and pH of 30ºC, 70% and 5 were determined following optimization. Using optimized parameters laboratory scale-up in static tray fermenter was performed that resulted in production of complete and balanced cellulolytic enzyme system. The balanced enzyme system had required 1:1 ratio of filter paper and beta-glucosidase units. This complete and balanced enzyme system was shown to be effective in the hydrolysis of wheat straw to sugars. Mild pretreatments– steam, acid and alkali were performed to vary physicochemical characteristics of soybean hulls – bed porosity, crystallinity and volumetric specific surface. Mild nature of pretreatments minimized the compositional changes of substrate. It was explicitly shown that more porous and crystalline steam pretreated soybean hulls significantly improved cellulolytic enzymes production in T. reesei culture, with no effect on xylanase. In A. oryzae and mixed culture this improvement, though, was not seen. Further studies using standard crystalline substrates and substrates with varying bed porosity confirmed that effect of physicochemical characteristics was selective with respect to fungal species and cellulolytic activity. A novel deep bed bioreactor was designed and fabricated to address scale-up issues. Bioreactor’s unique design of outer wire mesh frame with internal air distribution and a near saturation environment within cabinet resulted in enhanced heat transfer with minimum moisture loss. Enzyme production was faster and leveled within 48 h of operation compared to 96 h required in static tray. A two phase heat and mass transfer model was written that accurately predicted the experimental temperature profile. Simulations also showed that bioreactor operation was more sensitive to changes in cabinet temperature and mass flow rate of distributor air than air temperature. Trichoderma reesei Aspergillus oryzae Crystallinity bed porosity Solid-state bioreactor N-tank in series model Food Science (0359)
254	The role of sucker wounds as portals for grapevine trunk pathogen infections Makatini, Gugulethu Joy 04 1900 (has links) Thesis (MScAgric)--Stellenbosch University, 2014. / ENGLISH ABSTRACT: Grapevine trunk diseases are responsible for reduced wine and table grape production world-wide. Trunk disease infections are caused by xylem-inhabiting pathogens which include species of Botryosphaeriaceae, Diatrypaceae, Hymenochaetales and Diaporthales, as well as Phaeomoniella chlamydospora and Phaeoacremonium spp. Winter pruning wounds are regarded as the main infection-sites for trunk disease pathogens. However, the role of sucker wounds as portals of trunk disease infections has been minimally investigated. Knowledge of the potential role of grapevine trunk pathogen infections that occur through sucker wounds is important for better wound protection strategies. The aim of this study was to determine the role of grapevine sucker wounds as portals of entry for trunk disease pathogens and to assess the use of Trichoderma spp. for sucker wound protection. The susceptibility of sucker wounds to different trunk disease pathogens was assessed from natural as well as artificial infections. In addition the duration of sucker wound susceptibility in the field was also ascertained. Sucker wounds were sampled from three wine and two table grape vineyards during 2011 and 2012 in the Western Cape province of South Africa. Thereafter, fungal isolations were made from 161 sucker wounds and the cultures were identified based on cultural and morphological characteristics as well as the internal transcribed spacer regions and 5.8S ribosomal RNA gene. Sixty-two percent of the wounds were naturally infected by at least one of the trunk pathogens. Phomopsis (Po.) viticola (46%; 18%), Diplodia (D.) seriata (30%; 9%) and Phaeomoniella (Ph.) chlamydospora (27%; 5%) were the most predominant trunk disease pathogens isolated from sucker wounds of field wine and table grape cultivars, respectively. Lower incidences of Phaeoacremonium aleophilum (18%), Eutypella sp. (3%), Cryptovalsa ampelina (2%), Diplodia sp. (1%) and Neofusicoccum australe (1%) were obtained, however, only from wine grapes. Sucker wounds on 1-year-old potted grapevine plants of Chardonnay cultivar were inoculated with spore suspensions of Eutypa lata, N. parvum, Pa. aleophilum, Ph. chlamydospora and Po. viticola in the glasshouse. After 4 months all the inoculated pathogens could be re-isolated at the following incidences: N. parvum (85%), Ph. chlamydospora (75%), Po. viticola (65%), Pa. aleophilum (55%) and E. lata (45%). Sucker wound susceptibility was further ascertained under field conditions on 12-year-old Cabernet Sauvignon vines by artificial inoculation of the same pathogen species. After 5 months three pathogens could be re-isolated at the following incidences: Po. viticola (65%), N. parvum (32.5%) and Ph. chlamydospora (7.5%). The duration of susceptibility of field sucker wounds to Ph. chlamydospora was assessed for a period of 4 weeks. The wounds remained susceptible for 4 weeks with a decline in susceptibility after one week. This study showed that sucker wounds are susceptible to the major trunk disease pathogens and thus could play an important role in grapevine trunk disease epidemiology. In the second part of this thesis a possible management strategy to prevent infections of sucker wounds was investigated. The use of Trichoderma (T.) harzianum against two trunk pathogens on sucker wounds was tested in the field. Additionally the sensitivity of T. harzianum and T. atroviride was tested in vitro against 16 fungicides that are used to control powdery mildew, downy mildew, Botrytis rot and Phomopsis cane and leaf spot. In October 2012, sucker wounds were made on 1-year-old wood of Cabernet Sauvignon and spray-treated with Eco-77® immediately after desuckering, and then inoculated with spore suspensions of either Ph. chlamydospora or Po. viticola after 24 hours. After 5 months, isolations were made from the sucker wounds to evaluate the efficacy of the Trichoderma treatment. Trichoderma harzianum reduced the incidence of Ph. chlamydospora by 66.65%. Although the incidence of Po. viticola was reduced by 15.37%, it was not significantly different from the control treatment. The inhibition of mycelial growth and conidial germination of T. harzianum and T. atroviride were screened against 16 fungicides. The fungicides were applied at 0, 0.25, 0.5, 1 and 2 times the recommended dosages. Systemic fungicides boscalid, metrafenone and trifloxystrobin, as well as contact fungicides quinoxyfen and meptyldinocap were least toxic to Trichoderma spp. isolates. For the conidial germination assay, boscalid, trifloxystrobin, penconazole and metrafenone (systemic) plus quinoxyfen and folpet (contact) were compatible with Trichoderma spp. These fungicides were regarded as being compatible with Trichoderma spp. isolates because they gave mean percentage inhibitions of less than 50% at all the tested dosages. Spiroxamine and pyrimethanil gave the highest mean percentage inhibitions for both mycelial inhibition and conidial germination. The findings of this study showed that T. harzianum can protect sucker wounds against Ph. chlamydospora in the field. Furthermore, some fungicides applied for the control of powdery mildew and Phomopsis cane and leaf spot can be alternatively or simultaneously applied with T. harzianum and T. atroviride, however, this will have to be verified with field trials. / AFRIKAANSE OPSOMMING: Wingerd stamsiektes is wêreldwyd verantwoordelik vir verminderde wyn- en tafeldruif produksie. Stamsiektes word veroorsaak deur patogene wat in die xileem voorkom, insluitend verskeie spesies in die Botryosphaeriaceae, Diatrypaceae, Hymenochaetales en Diaporthales, asook Phaeomoniella chlamydospora en Phaeoacremonium spp. Winter snoeiwonde word beskou as die hoof bron van infeksies vir stamsiekte patogene. Die rol van suierwonde as poorte van infeksie vir stamsiektes is nog nie goed bestudeer nie. Kennis van die potensiële rol van wingerd stamsiekte patogeen infeksies wat deur suierwonde plaasvind is belangrik vir die formulasie van beter wondbeskerming strategieë. Die mikpunt van hierdie studie was om die rol van suierwonde as ingangsportale vir wingerd stamsiekte patogene te bepaal en om die gebruik van Trichoderma spp. vir suierwond beskerming te evalueer. Die vatbaarheid van suierwonde vir verskillende stamsiekte patogene is geëvalueer vanuit natuurlike, sowel as kunsmatige infeksies. Die duur van suierwond vatbaarheid in die veld is ook bepaal. Suierwonde is versamel vanuit drie wyn- en twee tafeldruif wingerde gedurende 2011 en 2012 in die Wes Kaap provinsie van Suid Afrika. Hierna is swam isolasies gemaak vanuit 161 suierwonde en die kulture is geïdentifiseer volgens kultuur en morfologiese kenmerke, sowel as die interne transkribeerde spasieerders en 5.8S ribosomale RNA geen. Twee-en-sestig persent van die wonde was geïnfekteer deur ten minste een van die stamsiekte patogene. Phomopsis (Po.) viticola (46%; 18%), Diplodia (D.) seriata (30%; 9%) en Phaeomoniella (Ph.) chlamydospora (27%; 5%) was die mees algemene stamsiekte patogene wat, respektiewelik, vanuit die wyn- en tafeldruif kultivars verky is. Laer hoeveelhede Phaeoacremonium aleophilum (18%), Eutypella sp. (3%), Cryptovalsa ampelina (2%), Diplodia sp. (1%) en Neofusicoccum australe (1%) is verkry, en slegs vanaf wyndruiwe. Suierwonde op 1-jaar oue Chardonnay wingerdplante in potte is in die glashuis geïnokuleer met spoorsuspensies van Eutypa lata, N. parvum, Pa. aleophilum, Ph. chlamydospora en Po. viticola. Na 4 maande kon al die geïnokuleerde patogene her-isoleer word teen die volgende hoeveelhede: N. parvum (85%), Ph. chlamydospora (75%), Po. viticola (65%), Pa. aleophilum (55%) en E. lata (45%). Suierwond vatbaarheid is verder geëvalueer onder veld kondisies op 12-jaar oue Cabernet Sauvignon plante deur kunsmatige inokulasie van die selfde patogeen spesies. Na 5 maande kon drie patogene her-isoleer word teen die volgende hoeveelhede: Po. viticola (65%), N. parvum (32.5%) en Ph. chlamydospora (7.5%). Die duur van vatbaarheid van suierwonde teen Ph. chlamydospora in die veld is geevalueer oor ‘n periode van 4 weke. Die wonde het vatbaar gebly vir 4 weke met ‘n afname in vatbaarheid na ‘n week. Hierdie studie demonstreer dat suierwonde vatbaar is vir die hoof wingerd stamsiektes en dus ‘n belangrike rol in die epidemiologie van wingerd stamsiektes kan speel. In die tweede deel van hierdie tesis is ‘n moontlike bestuurs-strategie ondersoek om infeksie van suierwonde te verhoed. Die gebruik van Trichoderma (T.) harzianum teen twee stampatogene op suierwonde is getoets in die veld. Verder is die in vitro sensitiwiteit van T. harzianum en T. atroviride getoets teen 16 fungisiedes wat gebruik word in die beheer van poeieragtige meeldou, donsskimmel, Botrytis vrot en Phomopsis streepvlek. Gedurende Oktober 2012 is suierwonde gemaak op 1-jaar oue hout van Cabernet Sauvignon en onmiddelik behandel met Eco-77® na suiering. Wonde is dan geïnokuleer met spoorsuspensies van óf Ph. chlamydospora óf Po. viticola na 24 uur. Na 5 maande is isolasies gemaak vanaf suierwonde om die doeltreffendheid van van die Trichoderma behandeling te evalueer. Trichoderma harzianum het die voorkoms van Ph. chlamydospora met 66.65% verminder. Alhoewel die voorkoms van Po. viticola verminder is met 15.37%, was dit nie ‘n beduidende verskil in vergelyking met die kontrole behandeling nie. Die inhibisie van miselium groei en konidia ontkieming van T. harzianum en T. atroviride is getoets teen 16 fungisiedes. Die fungisiedes is aangewend teen 0, 0.25, 0.5, 1 en 2 keer die aanbevole dosisse. Sistemiese fungisiedes boscalid, metrafenone en trifloxystrobin, sowel as kontak fungisiedes quinoxyfen en meptyldinocap was die minste toksies teen Trichoderma spp. Gedurende die konidia ontkiemingstoets was boscalid, trifloxystrobin, penconazole en metrafenone (sistemies) en quinoxyfen en folpet (kontak) versoenbaar met Trichoderma spp. Die fungisiedes is beskou as bruikbaar met Trichoderma spp. isolate omdat hulle gemiddelde persentasie inhibisies van minder as 50% teen al die getoetste dosisse gelewer het. Spiroxamine en pyrimethanil het die hoogste gemiddelde persentasie inhibisie gelewer vir beide die miselium inhibisie en konidia ontkieming. Die bevindings van hierdie studie het gewys dat T. harzianum suierwonde kan beskerm teen Ph. chlamydospora in die veld. Verder sou sommige fungisiedes wat aangewend word vir die bestuur van poeieragtige meeldou en streepvlek moontlik alternatiewelik of gelyktydig met T. harzianum en T. atroviride aangewend word, alhowel dit met veldproewe bevestig moet word. Grapevine trunk diseases Pruning wounds UCTD Theses -- Plant pathology Dissertations -- Plant pathology
255	Transporte de glicose em Trichoderma reesei: caracterização estrutural e funcional dos genes Trhxt1 e Trhxt2 / Glucose transport in Trichoderma reesei: structural and functional characterization of the Trhxt1 and Trhxt2 genes Ramos, Augusto Savio Peixoto 05 November 2002 (has links) O fungo filamentoso Trichoderma reesei é caracteristicamente reconhecido pela produção de celulases e hemicelulases, que lhe permitem utilizar uma ampla variedade de polissacarídeos como fonte de carbono. Neste trabalho, descrevemos a caracterização de dois genes de T. reesei, Trhxt1 e Trhxt2, que codificam proteínas com alta similaridade a transportadores de glicose de vários microorganismos. Os dois genes foram identificados em um banco de dados de ESTs de T. reesei. A análise computacional de Trhxt1 e Trhxt2 indica que ambos fazem parte da major facilitator superfamily (MFS), apresentando, tipicamente, 12 segmentos transmembrânicos. A expressão de Trhxt1 ocorre apenas em baixos níveis de glicose(≈ 100 µmol 1-1), enquanto a de Trhxt2 parece ocorrer de forma constitutiva, independentemente da fonte de carbono. Em baixas concentrações de oxigênio, a expressão de Trhxt1 é induzida e a de Trhxt2, reprimida. O sistema de transporte em T. reesei apresenta um componente de afinidade muito alta por glicose (Km ≈ 20 µmol 1-1) semelhante ao de outros fungos filamentosos. Dados sobre o transporte de glicose em uma cepa mutante ΔTrhxt1 indicam que o gene Trhxt1 está envolvido com o transporte em baixos níveis de glicose (≤ 100 µmol 1-1) que correspondem, provavelmente, aos valores encontrados no solo, o habitat natural de T. reesei.. Interessantemente, a indução do sistema de celulases de T. reesei por celulose está retardada no mutante ΔTrhxt1, o que sugere a importância do transporte de glicose na expressão dos genes das celulases. Finalmente, além de descrever os primeiros genes de transportadores de glicose em T. reesei, esperamos que este trabalho possa contribuir para o preenchimento de uma lacuna em relação ao transporte de açúcares em fungos filamentosos em geral. / The filamentous fungus Trichoderma reesei is a natural soil inhabitant capable of metabolizing a vast number of polysaccharide substrates. In this work, we describe two genes of T. reesei, named Trhxt1 and Trhxt2, which code for proteins with significant similarities to glucose transporters from other fungi. These genes were identified in an EST database of T. reesei. Sequence analysis of TrHXT1 and TrHXT2 revealed 12 putative transmembrane domains and several other characteristic motifs found in members of the major facilitator superfamily (MFS). Trhxt1 is transcriptionally induced only by low levels of glucose(≈ 100 µmol 1-1), while Trhxt2 expressionis independent of both glucose concentration and carbon source. We also show that Trhxt1 expression is enhanced when cells are exposured to low oxygen levels; in contrast, Trhxt2 expression seems to be repressed at these conditions. Glucose transport in T. reesei is apparently mediated by a multicomponent uptake system, in which the high-affiníty component has a Km of approximately 20 µmol 1-1. This low Km value is similar to the values reported for glucose uptake by other filamentous fungi. Kinetics of glucose transport in a T. reesei ΔTrhxt1 strain suggests that Trhxt1 is involved in glucose uptake in conditions of low glucose (≤ 100 µmol 1-1), which are most probably found in the soil, a low-nutrient environment. Interestingly, índuction ofthe T. reesei cellulase system by cellulose ís significantly delayed in the ΔTrhxt1 mutant, suggesting that glucose transport may be important to the mechanisms of expression of the cellulase genes. Finally, we hope that this work may be helpful to provide a better understanding of sugar uptake in filamentous fungi, for which there is little information available. Expressão gênica Filamentous fungus Fungo filamentoso Gene expression Glicose Glucose Glucose transport Hexose Hexose Membrana plasmática Transporte de glicose Trichoderma
256	Caracterização genética e citológica da recombinação somática em Trichoderma pseudokoningii. / Genetic and cytological characterization of the somatic recombination in Trichoderma pseudokoningii. Barcellos, Fernando Gomes 28 August 2002 (has links) Com o objetivo de se caracterizar o processo de recombinação somática em Trichoderma pseudokoningii foram feitos cruzamentos via anastomose de hifas entre duas linhagens contrastantes para quatro marcadores de auxotrofia, coloração dos conídios e marcadores de RAPD. Foram feitos quatro cruzamentos, sendo analisados um total de 1052 colônias obtidas a partir de suspensões de conídios provenientes das colônias heterocarióticas. Sessenta e oito colônias recombinantes foram analisadas quanto às marcas de auxotrofia em quatro gerações de crescimento, sendo observado que 58 mantiveram o fenótipo recombinante, enquanto que as colônias restantes reverteram para um dos parentais. A maioria das colônias recombinantes se mostrou instável. Entretanto, após 4 gerações de crescimento estas colônias se tornaram estáveis para as marcas de auxotrofia avaliadas. As colônias recombinantes instáveis apresentaram bordas de crescimento irregular, esporulação esparsa e a freqüente formação de setores. Estas colônias recombinantes foram analisadas quanto aos marcadores RAPD, tendo mostrado grande similaridade, em relação ao perfil de bandas apresentado, com a maioria dos primers analisados. Somente com um primer foi possível visualizar a presença de uma banda polimórfica entre os recombinantes e a presença de bandas nos parentais não existentes em alguns recombinantes. Cinco colônias recombinantes foram analisadas quanto ao perfil de bandas cromossomais (PFGE), tendo sido observado que 2 colônias apresentaram padrões cromossomais igual a um dos parentais e 3 colônias apresentaram padrões recombinantes. Nos estudos citológicos verificou-se a formação de conídios uninucleados na conidiogênese, e a presença de conídios verdes maduros multinucleados, devido a prováveis divisões nucleares durante o processo de maturação dos conídios. Observou-se durante a formação dos heterocários a ocorrência de anastomoses e a passagem de núcleos, tendo sido observado a presença de núcleos com várias conformações, sugerindo um movimento ativo dos mesmos. Os resultados acima sugerem a ocorrência de mecanismos de recombinação no heterocário (recombinação somática), diferentes daqueles descritos para o ciclo parassexual ou parameiose, sendo proposto a ocorrência da degradação, no heterocário, dos núcleos de um dos parentais envolvidos nos cruzamentos (parental não prevalente) e a incorporação de segmentos destes em núcleos íntegros do parental prevalente. Se estes eventos realmente estiverem ocorrendo, sugere-se que estes sejam devido a possíveis reações limitadas de incompatibilidade vegetativa, ocasionando processos de lise e morte celular em algumas regiões do micélio heterocariótico. / To understand the somatic recombination process in Trichoderma pseudokoningii, auxotrophic complementary mutant strains were used to produce 4 heterokaryons. These strains were contrasting for four auxotrophic markers, conidia colors and for some RAPD markers. It was analyzed a total of 1052 colonies obtained from conidial suspensions of the heterokaryotic colonies. Stability of auxotrophic markers was evaluated in 68 recombinant colonies after four growing generations. In this analysis, 58 colonies kept the recombinant phenotype, while 10 reverted to one parental strain. Most of the recombinant colonies were initially unstable, but after at least 4 growing generations these recombinants became stable for auxotrophic markers. The unstable recombinant colonies showed irregular growing borders, sparse sporulation and frequent sector formation. The recombinant colonies were analyzed by RAPD technique. These colonies showed high similarity for the most of used primers. However, one primer showed a polymorphic band and some recombinants missing bands observed in parental strains. Chromosomal band profile of 5 recombinants and two parental strains were analyzed by Pulsed Field Gel Electrophoresis technique (PFGE). Two recombinants showed parental profiles and 3 showed recombinant profiles, respectively. In cytological studies of the conidiogenesis was observed the formation of only uninucleated conidia. However, presence of multinucleated mature green conidia was evident, probably due to nuclear divisions in course of maturing process of the conidia. During the process of heterokaryotic mycelium formation was possible to observe the occurrence of anastomosis that showed nuclear transfer. The presence of nuclei in several conformations was observed at the different regions of the heterokaryon, suggesting an active movement. The results presented in this study suggest the occurrence of recombination mechanisms in the heterokayon (somatic recombination), different from those described in classic parasexual cycle or parameiosis. Thus, it was proposed that may occur during this recombinant process the degradation of nuclei from one parental (non-prevalent parental) in the heterokaryon, and that the resulting chromosomal fragments may be incorporated into whole nuclei of the another parental (prevalent parental). If this natural transformation is occurring during this recombination process could be suggested that this event is due to a limited incompatible vegetative reactions, generating cellular lyses and death in some regions of the heterokaryotic mycelium. cellulolytic fungus ciclo parassexual fungo celulolítico genética microbiana microbial genetics mitotic recombination parasexual cycle recombinação mitótica trichoderma
257	Estudos bioquímicos e moleculares de genes de trichoderma envolvidos no mecanismo de micoparasitismo Siqueira, Saulo José Linhares de 30 March 2012 (has links) Submitted by Marlene Santos (marlene.bc.ufg@gmail.com) on 2014-10-10T21:54:56Z No. of bitstreams: 2 Tese - Saulo José Linhares de Siqueira - 2012.pdf: 3918109 bytes, checksum: cfb7931590a50ed74838d6c8cefab1ee (MD5) license_rdf: 23148 bytes, checksum: 9da0b6dfac957114c6a7714714b86306 (MD5) / Approved for entry into archive by Jaqueline Silva (jtas29@gmail.com) on 2014-10-13T20:44:05Z (GMT) No. of bitstreams: 2 Tese - Saulo José Linhares de Siqueira - 2012.pdf: 3918109 bytes, checksum: cfb7931590a50ed74838d6c8cefab1ee (MD5) license_rdf: 23148 bytes, checksum: 9da0b6dfac957114c6a7714714b86306 (MD5) / Made available in DSpace on 2014-10-13T20:44:05Z (GMT). No. of bitstreams: 2 Tese - Saulo José Linhares de Siqueira - 2012.pdf: 3918109 bytes, checksum: cfb7931590a50ed74838d6c8cefab1ee (MD5) license_rdf: 23148 bytes, checksum: 9da0b6dfac957114c6a7714714b86306 (MD5) Previous issue date: 2012-03-30 / Species of Trichoderma are commercially applied as biological control agents and are antagonists of important plant pathogenic fungi (as Rhizoctonia, Sclerotinia and Fusarium species) due to its mycoparasitic characteristics. Research has been performed to have a better comprehension of molecular aspects of the biocontrol mechanisms performed by Trichoderma and to find isolates with high antagonistic potential against plant pathogens. In the present study the expression of mycoparasitism-related genes was performed T. asperellum T00 and T. harzianum ALL42 (Enzimologia group ICB/UFG fungal collection) that have great potential as biocontrol agent. Each chapter of this work refers to one of the species studied. In Chapter 1 T. asperellum isolate T00, known to produce high levels of cell wall degrading enzymes, has its β-1,3-glucanases enzymes and genes (tag83 and tag27) studied. The gene tag27 was cloned and characterized and codes to an 27kDa endo-β-1,3glucanase with and 285 aminoacids and 96% similar to a glucanases from T.atroviride. The enzyme was detected when T. asperellum was grown in Rhizoctonia solani or Sclerotinia sclerotiorum cell wall-containing media but not in Fusarium oxysporum cell wall-containing media. The tag83 and tag27 genes was repressed in media containing glucose as carbon source and upregulated in cell wall containing media and during plate confrontation tests with pathogenic fungi. Chapter 2 shows T. harzianum isolate ALL42 genes involved in mycoparasitism against R. solani or S. sclerotiorum detected using subtractive hybridization approach. T. harzianum was grown with R. solani or S. sclerotiorum cell wall as carbon source and the RNA used both as tester and driver in each of two subtractive library constructed. Sequencing analysis resulted in 47 genes related with growth in R. solani cell wall media and 114 genes related with growth in S. sclerotiorum cell wall media. To confirm the obtained data, 18 genes were tested by quantitative real time RT-PCR and 9 were differentially expressed in the same condition of the library they were detected. Five of these genes were also differentially expressed during plate confrontation assay with the respective pathogen, two of them expressed during contact with R. solani (cutinase and alginate lyase) and 3 during contact with S. sclerotiorum (hsp98, serin endopeptidase and a hypotetic gene). The results presented in this study provides additional information about the role of 1,3glucanase genes in mycoparasitism and of other genes related to antagonism against specific pathogens, providing helpful insights in the mechanism of biocontrol performed by Trichoderma. / Espécies do gênero Trichoderma são eficientes antagonistas de fungos fitopatogênicos, como as espécies Rhizoctonia, Sclerotinia e Fusarium, e são comercializados como agentes de controle biológico principalmente por sua característica de micoparasita. Muitos estudos têm sido feitos para compreender as bases moleculares dos mecanismos de biocontrole de Trichoderma e também para encontrar espécies com alto potencial de antagonismo contra fitopatógenos. O objetivo deste trabalho foi analisar a expressão de genes relacionados ao micoparasitismo de T. asperellum T00 e T. harzianum ALL42 (Enzimologia ICB/UFG) que possuem potencial para uso como agente de biocontrole. Este trabalho foi dividido em dois capítulos. O Capítulo 1 se refere ao fungo T. asperellum T00 e suas β-1,3-glicanases (TAG83 e TAG27) que degradam componentes da parede celular de fungos fitopatógenos. O gene tag27 codifica para uma endo-β-1,3glicanase de 27kDa que possui 285 resíduos de aminoácidos e apresentou 96% de similaridade com uma enzima de T. atroviride. A enzima foi secretada em meio de cultura contendo parede celular de Rhizoctonia solani e Sclerotinia sclerotiorum, mas não em meio com parede de Fusarium oxysporum. A expressão dos genes tag83 e tag27 foi reprimida na presença de glicose e ativada tanto na presença de parede celular dos fitopatógenos quanto durante o contato entre os fungos em placa. O Capítulo 2 trata do fungo T. harzianum isolado ALL42 e de genes identificados pela técnica de hibridização subtrativa relacionados especificamente ao biocontrole contra R. solani e S. sclerotiorum. Foram construídas duas bibliotecas subtrativas sendo que os RNAs utilizados como condição teste e controle da subtração foram obtidos de T. harzianum crescido em meio contendo parede celular de R. solani ou S. sclerotiorum. As bibliotecas foram sequenciadas resultando em 47 genes relacionados ao crescimento em meio com R. solani e 114 genes relacionados ao crescimento em meio com S. sclerotiorum. Dos 18 genes escolhidos para validação da biblioteca por RT-PCR em tempo real, 9 se mostraram diferencialmente expressos na condição correspondente à biblioteca em que foram identificados. Dentre estes, 5 genes se mostraram também diferencialmente expressos em experimento de confronto em placa, 2 deles mais expressos contra R. solani (cutinase e alginato liase) e 3 contra S. sclerotiorum (hsp98, serina endopeptidase e um de função hipotética). Os resultados obtidos com as duas linhagens fornecem informações adicionais sobre genes de β-1,3-glicanases, conhecidamente envolvidos no processo de micoparasitismo, e sobre genes relacionados ao antagonismo de patógenos específicos, além de contribuir para o conhecimento relacionado ao biocontrole realizado por fungos do gênero Trichoderma. Trichoderma Micoparasitismo β-1,3-glicanases Bibliotecas subtrativas Mycoparasitism β-1,3-glucanases Subtractive hybridization MORFOLOGIA::CITOLOGIA E BIOLOGIA CELULAR
258	Functional studies and engineering of family 1 carbohydrate-binding modules Lehtiö, Janne January 2001 (has links) The family 1 cellulose-binding modules (CBM1) form a groupof small, stable carbohydrate-binding proteins. These modulesare essential for fungal cellulosedegradation. This thesisdescribes both functional studies of the CBM1s as well asprotein engineering of the modules for several objectives. The characteristics and specificity of CBM1s from theTrichoderma reeseiCel7A and Cel6A, along with severalother wild type and mutated CBMs, were studied using bindingexperiments and transmission electron microscopy (TEM). Datafrom the binding studies confirmed that the presence of onetryptophan residue on the CBM1 binding face enhances itsbinding to crystalline cellulose. The twoT. reeseiCBM1s as well as the CBM3 from theClostridium thermocellumCipA were investigated by TEMexperiments. All three CBMs were found to bind in lineararrangements along the sides of the fibrils. Further analysesof the bound CBMs indicated that the CBMs bind to the exposedhydrophobic surfaces, the so called (200) crystalline face ofValoniacellulose crystals. The function and specificity of CBM1s as a part of an intactenzyme were studied by replacing the CBM from the exo-actingCel7A by the CBM1 from the endoglucanase Cel7B. Apart fromslightly improved affinity of the hybrid enzyme, the moduleexchange did not significantly influence the function of theCel7A. This indicates that the two CBM1s are analogous in theirbinding properties and function during cellulosehydrolysis. The CBM1 was also used for immobilization studies. Toimprove heterologous expression of a CBM1-lipase fusionprotein, a linker stability study was carried out inPichia pastoris. A proline/threonine rich linker peptidewas found to be stable for protein production in this host. Forwhole bacterial cell immobilization, theT. reeseiCel6A CBM1 was expressed on the surface of thegram-positive bacteria,Staphylococcus carnosus. The engineeredS. carnosuscells were shown to bind cellulosefibers. To exploit the stable CBM1 fold as a starting point forgenerating novel binders, a phage display library wasconstructed. Binding proteins against an amylase as well asagainst a metal ion were selected from the library. Theamylase-binding proteins were found to bind and inhibit thetarget enzyme. The metal binding proteins selected from thelibrary were cloned on the surface of theS. carnosusand clearly enhanced the metal bindingability of the engineered bacteria. <b>Keywords</b>: cellulose-binding, family 1carbohydrate-binding module, phage display, bacterial surfacedisplay, combinatorial protein library, metal binding, proteinengineering,Trichoderma reesei, Staphyloccus carnosus. Cellulose-binding carbohydrate-binding modules phage display bacterial surface display combinatorial protein library protein engineering Trichoderma reesei Staphylococcus carnosus
259	Functional studies and engineering of family 1 carbohydrate-binding modules Lehtiö, Janne January 2001 (has links) <p>The family 1 cellulose-binding modules (CBM1) form a groupof small, stable carbohydrate-binding proteins. These modulesare essential for fungal cellulosedegradation. This thesisdescribes both functional studies of the CBM1s as well asprotein engineering of the modules for several objectives.</p><p>The characteristics and specificity of CBM1s from the<i>Trichoderma reesei</i>Cel7A and Cel6A, along with severalother wild type and mutated CBMs, were studied using bindingexperiments and transmission electron microscopy (TEM). Datafrom the binding studies confirmed that the presence of onetryptophan residue on the CBM1 binding face enhances itsbinding to crystalline cellulose. The two<i>T. reesei</i>CBM1s as well as the CBM3 from the<i>Clostridium thermocellum</i>CipA were investigated by TEMexperiments. All three CBMs were found to bind in lineararrangements along the sides of the fibrils. Further analysesof the bound CBMs indicated that the CBMs bind to the exposedhydrophobic surfaces, the so called (200) crystalline face of<i>Valonia</i>cellulose crystals.</p><p>The function and specificity of CBM1s as a part of an intactenzyme were studied by replacing the CBM from the exo-actingCel7A by the CBM1 from the endoglucanase Cel7B. Apart fromslightly improved affinity of the hybrid enzyme, the moduleexchange did not significantly influence the function of theCel7A. This indicates that the two CBM1s are analogous in theirbinding properties and function during cellulosehydrolysis.</p><p>The CBM1 was also used for immobilization studies. Toimprove heterologous expression of a CBM1-lipase fusionprotein, a linker stability study was carried out in<i>Pichia pastoris</i>. A proline/threonine rich linker peptidewas found to be stable for protein production in this host. Forwhole bacterial cell immobilization, the<i>T. reesei</i>Cel6A CBM1 was expressed on the surface of thegram-positive bacteria,<i>Staphylococcus carnosus</i>. The engineered<i>S. carnosus</i>cells were shown to bind cellulosefibers.</p><p>To exploit the stable CBM1 fold as a starting point forgenerating novel binders, a phage display library wasconstructed. Binding proteins against an amylase as well asagainst a metal ion were selected from the library. Theamylase-binding proteins were found to bind and inhibit thetarget enzyme. The metal binding proteins selected from thelibrary were cloned on the surface of the<i>S. carnosus</i>and clearly enhanced the metal bindingability of the engineered bacteria.</p><p><b>Keywords</b>: cellulose-binding, family 1carbohydrate-binding module, phage display, bacterial surfacedisplay, combinatorial protein library, metal binding, proteinengineering,<i>Trichoderma reesei, Staphyloccus carnosus</i>.</p> Cellulose-binding carbohydrate-binding modules phage display bacterial surface display combinatorial protein library protein engineering Trichoderma reesei Staphylococcus carnosus
260	Use of a commercially available Trichoderma spp. as a growth promoter for Sorghum bicolor l. moench growing on contaminated soil. Memel, Akpa Omer. January 2013 (has links) M. Tech. Chemistry / Aims to assess the viability of using Eco-T as a growth promoter in soils contaminated with different concentrations of As and Cu. Dissertations, Academic -- South Africa. Sorghum. Trichoderma. Soil pollution -- South Africa. Arsenic. Copper.

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