The Effects of Dixie Harrow Treatments on Greater Sage-grouse Resource Selection and the Nutritional Value of Sagebrush During Winter

Wood, Jason Alan

01 April 2019

Sagebrush (Artemisia spp.) is an important source of food and cover for many animals, especially during winter months. Understanding how wildlife species respond to sagebrush management actions can help improve conservation planning. Dixie harrow is a method of improving spring/summer habitat for many herbivores by reducing sagebrush cover to stimulate the growth of grasses and forbs. These treatments, however, may influence the quantity and quality of sagebrush available to greater sage-grouse (Centrocercus urophasianus; hereafter, sage-grouse) during winter. We evaluated the effects of Dixie harrow on sage-grouse resource selection during winter (Chapter 1) and on the nutritional value of sagebrush (Chapter 2). We were unsure what effect Dixie harrow would have on the nutritional value of sagebrush, but hypothesized that sage-grouse would select for untreated areas because they contained a higher quantity of food and cover. We captured 81 sage-grouse and fit them with GPS transmitters. Using 6,728 winter locations, we modeled third-order resource selection. Further, we collected samples of sagebrush plants that sage-grouse had eaten from (n = 54), samples of sagebrush plants passed by but not eaten from (n = 54), as well as samples from random locations inside (n = 60) and outside Dixie harrow treatments (n = 60). Contrary to our hypothesis, sage-grouse selected for Dixie harrow treatments during winter. We found that sage-grouse selectively browsed sagebrush plants with increased nutritional value, and that sage-grouse browsed plants inside treatments more frequently than outside the treatments, but Dixie harrow treatments had no measurable effect on the nutritional value of sagebrush. Based on our results, Dixie harrow treatments performed at the southern extent of the sage-grouse range will create habitat that sage-grouse prefer during winter, but we were unable to ascertain why sage-grouse select for Dixie harrow treatments during winter.

Dixie harrow

sagebrush

Grass Valley

greater sage-grouse

primary metabolite

secondary metabolite

resource selection

Life Sciences

Plant Sciences

Mise au point d'un bioréacteur de fermentation en milieu solide fonctionnant en continu pour la production de métabolites secondaires antioxydants par Aspergillus niger G131 / Development of a continuous pilote-scaled bioreactor for the production of antioxidant secondary metabolites by Aspergillus niger G131 using solid state fermentation

Carboué, Quentin

04 June 2018

Aspergillus niger souche G131 est un champignon qui produit en quantité des métabolites secondaires appartenant à la famille des naphtho-gamma-pyrones (NγPs). Ces NγPs sont des pigments qui présentent des intérêts industriels de par leurs importants potentiels antiradicalaires. L’objectif de ce doctorat est la production à l’échelle pilote et en continu de NγPs à travers la culture du champignon sur milieu solide. Le choix de la fermentation en milieu solide (FMS) comme processus de culture repose sur des aspects d’ordre qualitatif et quantitatif de production, ainsi que sur des raisons économiques et éthiques, relatives à la protection de l’environnement avec notamment la possibilité de valoriser des coproduits agricoles comme milieu de culture pour le champignon. Dans un premier temps, ce travail s’intéresse à la caractérisation de la composition et des potentialités associées aux molécules produites par la souche. Ces potentialités incluent les activités anti-radicalaires et les mesures de cytotoxicité. La thèse porte également sur la caractérisation de la physiologie de croissance de la souche en FMS et sur l’optimisation des conditions de culture par la méthodologie des plans d’expériences pour l’augmentation de la production de NγPs. Une stratégie originale d’optimisation adaptée aux contraintes posées par la FMS est d’ailleurs proposée. Finalement, un transfert d’échelle de production est réalisé au moyen d’un bioréacteur prototype innovant permettant la production à l’échelle pilote de milieu fermenté en continu. Dans son dernier chapitre, ce travail s’intéresse donc à la mise au point des paramètres opératifs qui entourent la production continue de NγPs par FMS. / Aspergillus niger strain G131 is a non-ochratoxigenic filamentous fungus producing high quantities of secondary metabolites known as naphtha-gamma-pyrones (NγPs). NγPs are pigments of industrial interest in reason of their high antioxidant properties. The aim of this dissertation is the continuous, pilote-scaled production of these NγPs through the cultivation of the fungus on solid medium. The choice of solid state fermentation (SSF) as cultivation method is not only driven by quantitative and qualitative considerations, but also by economical and ethical concerns related to environmental protection. SSF allows, in fact, a direct valorization of agricultural byproducts as the solid medium for the fungal growth. First, this work deals with the characterization of the composition and potentialities associated with the molecules produced by the strain, which include antioxidant and cytotoxic activities. Second, the dissertation focuses on the characterization of the fungal growth’s physiology on solid medium and on the optimization of the culture conditions using experimental methodology in order to increase NγPs production. For this purpose, an original optimization strategy is proposed to overcome specific constraints connected to SSF. Finally, a scale transfer of the production is advanced by means of an innovative prototype bioreactor continuously producing fermented material. The final chapter of this work addresses the development of parameters regarding the continuous NγPs production using SSF.

Fermentation en milieu solide

Bioréacteur

Aspergillus niger

Métabolite secondaire

Naphtho-Gamma-Pyrones

Antioxydant

Solid state fermentation

Bioreactor

Aspergillus niger

Secondary metabolite

Naphtha-Gamma-Pyrones

Antioxidant

\"Produção de metabólitos antimicrobianos e sideróforos de isolados provenientes de Terra Preta Antropogênica da Amazônia Ocidental\" / Antimicrobial metabolites and siderophore produced by strains from Anthropogenic Dark Earth of the Occidental Amazon

Fedrizzi, Samanta Maria Gobbo

30 November 2006

Os microrganismos atraem considerável atenção por serem uma fonte de compostos biotecnológicos e farmacêuticos. Diversos produtos naturais peptídicos produzidos por fungos e bactérias são sintetizados por grandes enzimas, conhecidas como peptídeo sintetase não ribossômica (NRPS) e policetídeo sintase (PKS). A bioprospecção dos microrganismos isolados do solo de Terra Preta Antropogênica (TPA) da Amazônia Ocidental é de grande importância para o conhecimento deste bioma tropical. Este estudo correlacionou a presença de sideróforos e de compostos antimicrobianos produzidos pelos microrganismos isolados de TPA e dos solos adjacentes com a presença dos genes que codificam para NRPS e PKS. Linhagens bacterianas foram isoladas das amostras do solo coletadas de 10, 20 e 40 cm de profundidade. Os isolados foram cultivados em meio líquido específico por 2 dias a 28oC. Um total de 143 isolados foi testado para a atividade de sideróforo e para isso, as linhagens foram inoculadas em um meio com baixa concentração de ferro (MM9) contendo o complexo cromoazurol S-Fe3. Do total, 72 isolados apresentaram reação positiva para a produção de sideróforo. O DNA genômico dos isolados foi extraído e a amplificação por PCR foi realizada usando iniciadores específicos para NRPS e PKS. Os resultados mostraram que quinze isolados apresentaram o gene que codifica para NRPS, vinte isolados para PKS e somente dez isolados apresentaram ambos os genes. A presença de genes de NRPS e PKS em 31% dos isolados testados sugere que a produção dos sideróforos possa ocorrer pela via não ribossomal. Dois isolados foram selecionados para estudos de identificação e caracterização dos compostos. O isolado TP11 foi identificado como Pseudomonas putida através de seqüenciamento do 16S rRNA e apresentou resultado negativo para hidroxamato e catecol, sugerindo que o tipo de sideróforo não possui nenhum destes grupos funcionais. O isolado TP16 foi identificado como Pseudomonas putida e apresentou produção de sideróforo do tipo catecol e hidroxamato, sugerindo a produção de mais de um sideróforo. Além disso, esta linhagem produziu um composto antimicrobiano, com atividade de sideróforo identificado por espectrometria de massas como pseudomonina com massa molar de 330 Da. / Microorganisms have attracted considerable attention as a source for biotechnological and pharmaceutical agents. Several peptidic natural products synthesized by fungi and bacteria are assembled by large enzymes, referred as nonribosomal peptide synthetase (NRPS) and polyketide synthase (PKS). Bioprospection of microorganisms isolated from Anthropological Dark Earth soil of Brazilian Occidental Amazon is of great importance to the knowledge of this tropical biome. This study aimed to correlate the presence of siderophores and antimicrobial compounds produced by microorganisms isolated from Dark Earth and adjacent soils of Brazilian Amazon with the presence of genes encoding NRPS and PKS. Bacterial strains were isolated from soil samples collected at 10, 20 and 40 cm depth. The isolates were grown in specific liquid medium for 2 d at 28oC. A total of 143 isolates were screened for siderophore activity and for this, bacterial strains were inoculated on plates containing an iron-limited medium (MM9) amended with a chromeazurol S-Fe3 complex. From the total, seventy-two isolates showed positive reaction for siderophore production. Genomic DNA of the isolates was extracted and PCR amplification was carried out using specific primers for NRPS and PKS. The results showed that fifteen isolates presented NRPS, twenty isolates presented PKS and only ten isolates showed both genes. The presence of NRPS and PKS genes in 31% of the isolates tested suggests that production of siderophores may occur by a nonribosomal pathway. Two isolates were selected for further studies. Isolate TP11 was identified as Pseudomonas putida by 16S rDNA sequencing analysis and was negative for hydroxamate and catechol, suggesting that the siderophore type has no hydroxamate- or catechol-type functional groups. The isolate TP16 was identified as Pseudomonas putida and showed the production of catechol and hydroxamate siderophore-type, suggesting the production of more than one siderophore. In addition, this strain produced an antimicrobial compound, with siderophore activity identified through mass spectrometry as pseudomonine with a molar mass of 330 Da.

16S rRNA

16S rRNA

Metabólito Secundário

Non-ribosomal Peptide Synthetase

Peptídeo Sintetase Não Ribossômica

Policetídeo Sintase

Polyketide Synthase

Pseudomonina.

Pseudomonine.

Secondary Metabolite

Bioprospecção de biomoléculas isoladas de fungos endofíticos de Combretum leprosum do bioma Caatinga / Bioprospection of biomolecule isolated from endophytic fungal of Combretum leprosum from Caatinga biome

Santos, Suikinai Nobre

03 September 2012

Os micro-organismos que habitam o interior das plantas (endofíticos ou endófitos) tornaram-se foco de interesse por estarem envolvidos na produção de compostos químicos como enzimas, alcalóides, antibióticos, anticancerígenas e diferentes metabólitos. Os ecossistemas de regiões tropicais tem sido alvo de busca de compostos naturais por causa da riqueza de espécies e nichos ecológicos presentes nestas comunidades. O objetivo deste trabalho o isolamento, identificação e a bioprospecção de fungos endofíticos obtidos de Combretum leprosum e a detecção nos extratos de planta e micro-organismos da presença do composto combretastatin (CA4). Folhas, galhos, frutos e raízes de C. leprosum foram coletados de cinco estados dentro da zona de semiárido brasileiro: Bahia, Piauí, Ceará, Paraíba, Rio Grande do Norte. Partes das amostras foram triturados e submetidos à maceração primeiramente em diclorometano, seguidos de tetrahidrofurano e acetona de acordo com Pettit et al.(1987) para possível extração da CA4. Além disso, para avaliação in vitro da atividade citotóxica e antimicrobiana foram realizadas extrações em acetato de etila, clorofórmio e metanol. Foram detectados a possível presença da CA4 em todos os órgãos das plantas extraídos com tetrahidrofurano e as maiores concentrações foram observadas nas folhas. A atividade antitumoral dos extratos vegetais apresentaram as maiores inibições contra carcinoma (ovário IC50 10µg/mL-1, rim IC50 8,7µg/mL-1 e mama IC50 14,1µg/mL-1) e glioma.IC50 13,5µg/mL-1. A outra parte das amostras (folhas, caules e raízes) foram desinfetadas, fragmentadas e colocadas em meios de cultivo (Martin, BDA, Agar água) por 60 dias, 28°C. Foram isolados 405 fungos endofíticos e 159 apresentaram atividade contra fitopatogênicos, 72% para Rhizoctonia solani e 28% para Pythium aphanidermatum. As vinte e três linhagens que apresentaram as melhores atividades antifitopatogênicas foram submetidas a crescimento em Czapec em cultura estacionaria, por 30 dias, a 28°C, os respectivos metabólitos foram obtidos em múltiplo (3.0 e 11.0) e avaliados a atividade antimicrobiana contra bactérias patogênicas e fungos. Quatro linhagens foram selecionadas, identificadas pelo sequenciamento da região 18S, CFE177 como Fusarium oxysporum, CFE03 como Hypocrea koningii, linhagem CFE108 como Aspesgillus oryzae e CFE391 como Fusarium solani e avaliadas in vitro pelos testes biológicos: atividade antitumoral, antioxidante e antimicobactéria. Os compostos produzidos por A. oryzae CFE108 apresentaram potencial para bioprospecção, e de acordo com as atividade citotóxicas as maiores ações foram contra as linhagens linfoma histiocística (J744), mieloma murino (B16F10) e baixa citotóxidade para carcinoma de bexiga (ECV304) e leucemia eritroblástica humana (k562) na concentração de 1mg/mL-1. Foram isolados dois compostos: SS-XL-32-01 identificado como bis-(2-etilhexil) ftalato (DEHP) e SS-XL-20-1 identificado como fenol, 2.2 metilenobis[6-(1,1-dimetiletil)-4- etil], ambos com atividade anticâncer para células HeLa com percentual de ate 98% e 71%, de morte, respectivamente. Alem disso, a modificação através da reação de metilação do composto SS-XL-32-1 resultou na quebra do anel aromático, formação de 4 subprodutos e perda da atividade, sendo um indicativo do sitio ativo da molécula responsável pela atividade observada. Portanto, fungos endofíticos de 18 plantas do semiárido brasileiro podem ser considerados fonte de bioprospecção para novas moléculas bioativas com atividade antitumoral. / The micro-organisms that reside in the aerial tissues and roots of plants (endophytic or endophyte) became the focus of interest for being involved in the chemical production such as enzymes, alkaloids, antibiotics, anticancer and different metabolites. The ecosystems of tropical region have been targeted search of natural compounds because of the richness of species and ecological niches present in these communities. The aim of this work was the isolation, identification and bioprospection for endophytic fungi from Combretum leprosum and detection in extracts of the plant and micro-organisms for the presence of the combretastatin (CA4). Leaves, stems, fruits and roots of C. leprosum were collected from five states within the semi-arid zone of Brazil: Bahia, Piaui, Ceara, Paraiba, Rio Grande do Norte. Part of the samples were crushed and subjected to maceration in dichloromethane, followed by tetrahydrofuran and acetone according to Pettit et al. (1987) for extracting the possible CA4. Moreover, for in vitro evaluation of the cytotoxic and antimicrobial activity extractions were carried out in ethyl acetate, chloroform and methanol. Were detected the possible presence of CA4 all plant organs extracted with tetrahydrofuran and the highest concentrations were observed on the leaves. The antitumor activity of plant extracts showed the highest inhibition against carcinoma (ovary IC50 10µg/mL-1, kidney IC50 8.7 µg/mL-1 and breast IC50 14.1 µg/mL-1) glioma IC50 and 13.5 mg-/mL-1. The other part of the samples (leaves, stems and roots) were disinfected, fragmented and placed in culture media (Martin, PDA, water agar) for 60 days, 28°C. 405 Endophytic fungi were isolated and 159 showed activity against phytopathogenic, 72% for Rhizoctonia solani and 28% for Pythium aphanidermatum. Twenty-three strains that showed good activities antiphytopathogenic, were grow on medium Czapec in static culture, for 30 days at 28°C, the respective metabolites were obtained in multiples pH (3.0 and 11.0) and evaluated the antimicrobial activity against pathogenic bacteria and fungi. Four strains were selected, identified by sequencing the 18S region, CFE177 as Fusarium oxysporum, CFE03 as Hypocrea koningii, strain CFE108 as Aspesgillus oryzae and CFE391 Fusarium solani, and evaluated by in vitro biological tests: antitumor, antioxidant and antimicobactérium activity. The compounds produced by A. oryzae CFE108 had biological potential and in accordance with the cytotoxic activity, showed the highest activities against lymphoma lines (J744), murine myeloma (B16F10) and low cytotoxicity for carcinoma of the bladder (ECV304) and leukemia erythroblastic human (K562) in 1mg/mL-1 concentration. Two compounds were isolated: SS-XL-32- 01 identified as bis-(2-ethylhexyl)phthalate (DEHP), and SS-XL-20-1 as phenol 2.2methylenobis [6-(1,1-dimethylethyl) - 4-ethyl], both with anticancer activity for HeLa cells with a percentage of up to 98% and 71%, of death, respectively. In addition, modified by methylation reaction of the compound SS-XL-32-1 resulted in the breaking of the aromatic ring and result in formation of four product and loss of activity being indicative of the active site of the molecule can be the aromatic ring. Therefore, endophytic fungi in semiarid Brazil plant can be considered a source of bioprospection for new bioactive molecules with anticancer activity.

Antitumor activity

Aspergillus oryzae

Aspergillus oryzae

Atividade antitumoral

Bioprospecção

Bioprospection

Caatinga

Caatinga

Combretum leprosum

Combretum leprosum

Endophytic fungi

Metabólitos secundários

Micro-organismos endofíticos

Secondary metabolite

Semiarid

Cyclodipeptide synthases : towards understanding their catalytic mechanism and the molecular bases of their specificity / Les cyclodipeptide synthases : vers la compréhension de leur mécanismecatalytique et des bases moléculaires de leur spécificité

Li, Yan

26 September 2012

Les cyclodipeptides et leurs dérivés, les dicétopipérazines (DKP), constituent une large classe de métabolites secondaires aux activités biologiques remarquables qui sont essentiellement synthétisés par des microorganismes. Les voies de biosynthèse de certaines DKP contiennent des synthases de cyclodipeptides (CDPS), une famille d’enzymes récemment identifiée. Les CDPS ont la particularité de détourner les ARNt aminoacylés de leur rôle essentiel dans la synthèse protéique ribosomale pour les utiliser comme substrats et ainsi catalyser la formation des deux liaisons peptidiques de différents cyclodipeptides. Le travail de thèse présenté dans ce manuscrit a pour objectif de caractériser la nouvelle famille des CDPS. Dans un premier temps, la caractérisation tant structurale que mécanistique de la première CDPS identifiée, AlbC de Streptomyces noursei, est présentée. Puis, les résultats obtenus avec trois autres CDPS, chacune de ces enzymes ayant des caractéristiques adéquates pour approfondir l’étude de la famille des CDPS, sont décrits. Ainsi, la CDPS Ndas_1148 de Nocardiopsis dassonvillei a permis d’étendre nos connaissances sur les bases moléculaires de la spécificité des CDPS. La CDPS AlbC-IMI de S. sp. IMI 351155 est un bon modèle pour analyser l’interaction de chacun des deux substrats nécessaires à la formation d’un cyclodipeptide. Enfin, la caractérisation de la CDPS Nvec-CDPS2 chez l’animal Nematostella vectensis a permis de fournir le premier exemple d’enzyme d’origine animale impliquée dans la synthèse peptidique non ribosomale. / Cyclodipeptides and their derivatives, the diketopiperazines (DKPs), constitute a large class of secondary metabolites with noteworthy biological activities that are mainly synthesized by microorganisms. The biosynthetic pathways of some DKPs contain cyclodipeptide synthases (CDPSs), a newly defined family of enzymes. CDPSs hijack aminoacyl-tRNAs from their essential role in ribosomal protein synthesis to catalyze the formation of the two peptide bonds of various cyclodipeptides. The aim of the work presented in this thesis manuscript is to characterize the CDPS family. At first, the structural and mechanistic characterization of the first identified CDPS, AlbC of Streptomyces noursei, is presented. Then, the results obtained with three other CDPSs, each of which having suitable properties to increase our understanding of the CDPS family, are described. The CDPS Ndas_1148 of Nocardiopsis dassonvillei extends our knowledge of the molecular bases of the CDPS specificity. The CDPS AlbC-IMI of S. sp. IMI 351155 is a good model to analyze the interaction of each of the two substrates required for the formation of a cyclodipeptide. Finally, the characterization of the CDPS Nvec-CDPS2 from Nematostella vectensis provides the first example of enzymes of animal origin involved in nonribosomal peptide synthesis.

Synthase de cyclodipeptide (CDPS)

Dicétopipérazine (DKP)

Biosynthèse nonribosomale

Liaison peptidique

ARNt aminoacylé

Métabolite secondaire

Cyclodipeptide synthase (CDPS)

Diketopiperazine (DKP)

Nonribosomal biosynthesis

Peptide bond

Aminoacyl-tRNA

Secondary metabolite

Caracterização de isolados de Sarocladium oryzae e seu potencial na supressão da brusone foliar em arroz / Characterization of Sarocladium oryzae isolates and their potential in the suppression of leaf blast in rice

Guimarães, Rafaela Araújo

21 August 2014

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No. of bitstreams: 2 Dissertação - Rafaela Araújo Guimarães - 2014.pdf: 1551849 bytes, checksum: b39011c17618c122fad17d142b0288ec (MD5) license_rdf: 23148 bytes, checksum: 9da0b6dfac957114c6a7714714b86306 (MD5) Previous issue date: 2014-08-21 / Conselho Nacional de Pesquisa e Desenvolvimento Científico e Tecnológico - CNPq / Sarocladium oryzae, the causal agent of rice sheath rot disease is described as antagonistic to rice pathogens. Rice blast is a major rice disease and is responsible for losses up to 100% in productivity. The disease control is done by integrated management, where the main practices are use of resistant cultivars and chemical control. The biocontrol agents or their metabolites may to be more practical to be including them as components in the management. The in objectives of this study a consist to evaluate of S. oryzae isolates for the morphological variability, genetics, biochemistry and antagonistic activity to rice pathogens; evaluate effect of S. oryzae filtrade on conidial germination and appressorium formation of M. oryzae; evaluate potential of conidia and filtrate S. oryzae in the suppression of leaf blast severity and quantify activity of enzymes involved in interaction M. oryzae x rice plant x S. oryzae. Isolates were characterized for color, texture, colony diameter, conidia size and hyphae thickness. In genetic studies, we used RAPD marker primers, and cerulenin production was quantified by HPLC. Antagonism in vitro was assessed by dual culture method. The effect of S. oryzae on conidial germination and appressorium formation of M. oryzae was evaluated using hydrophobic surface. Rice cultivar BRS Primavera, M. oryzae isolate (Py 10.900) and S. oryzae, isolate So 03, were utilized to study plant-pathogen-antagonist relationship. Plants were sprayed, with conidial suspension (CS), 3x105 conídios.mL-1 and culture filtrate (CF) 100% of S. oryzae, two days before inoculation with M. oryzae. S. oryzae isolates showed morphological variability, polymorphism in DNA. A majority of S. oryzae isolates (60%) ware able to produce cerulenin and over 55% were antagonistic to C. miyabeans, M. oryzae, M. albescens and T. cucumeris. The isolate So 29 showed largest inhibition zone. Filtrate of isolates So 03 and So 29 delayed conidia germination by 89.5% and inhibited appressoria formation of M. oryzae by 85%. CS reduced of leaf blast severity in 68.8% and CF in 75.5%. The enzymes β-1,3-glucanase and peroxidase exhibited maximum activity in plants sprayed with CF, when as the activity was high for SA and lipoxygenase in relation to CS treatment, compared to their respective controles, in the absence of M. oryzae. After inoculation with M. oryzae, the lipoxygenase and phenylalanine ammonia-lyase activity in both treatments CF and CS, showed differences compared to controls (plants inoculated with M. oryzae and water only). S. oryzae presented variability to characteristics evaluated and showed potential antagonism against to rice pathogens. Changes in enzyme activity indicate their role in induction resistance in plants in M. oryzae x rice x S. oryzae interaction. / Sarocladium oryzae, agente causal da podridão da bainha do arroz, é descrito como antagonista a patógenos de arroz. A brusone, principal doença do arroz é responsável por perdas de até 100% na produtividade. O controle desta doença é feito pelo uso do manejo integrado, onde as principais práticas são o uso de cultivares resistentes e o controle químico. O uso de agentes de biocontrole ou seus metabólitos pode ser mais uma prática a ser inserida ao manejo. Os objetivos deste estudo foram: avaliar isolados de S. oryzae quanto à variabilidade morfológica, genética, bioquímica e quanto à atividade antagônica aos patógenos de arroz; avaliar o efeito do filtrado de S. oryzae na germinação de conídios e na formação de apressórios de M. oryzae; avaliar o potencial da suspensão de conídios e do filtrado de S. oryzae na supressão da brusone foliar e quantificar a atividade das enzimas relacionadas à patogênese e do fitohormônio ácido salicílico (AS) envolvidos na interação M. oryzae x arroz x S. oryzae. Os isolados foram caracterizados quanto à cor, textura, diâmetro da colônia, tamanho dos conídios e espessura das hifas. No estudo genético, utilizou-se marcador RAPD (Random Amplified Polymorphic DNA) e a produção de cerulenina foi quantificada em HPLC. O antagonismo in vitro foi avaliado pelo método da cultura pareada. A ação de S. oryzae sobre a germinação de conídios e a formação de apressórios de M. oryzae foi avaliada em superfície hidrofóbica. Plantas de arroz da cultivar BRS Primavera, um isolado virulento de M. oryzae (Py 10.900) e o isolado So 03 de S. oryzae, foram avaliados no estabelecimento das relações planta-patógeno-antagonista. As plantas foram pulverizadas com S. oryzae, na forma de suspensão de conídios (SC) - 3x105 conídios.mL-1 e filtrado (FI) 100% concentrado, dois dias antes da inoculação com M. oryzae. Os isolados de S. oryzae apresentaram variabilidade morfológica e polimorfismo no DNA. A maioria dos isolados de S. oryzae (60%) foi capaz de produzir cerulenina e mais de 55% foram antagônicos a C. miyabeans, M. oryzae, M. albescens e T. cucumeris. O isolado So 29 apresentou o maior halo de inibição no pareamento. Os filtrados dos isolados So 03 e So 29 retardaram a germinação dos conídios em 89,5% e inibiram a formação dos apressórios de M. oryzae em 85%. A SC reduziu a severidade da brusone foliar em 68,8% e o FI em 75,5%. Os maiores valores de atividade enzimática específica em relação ao controle antes da presença de M. oryzae foram para β-1,3-glucanase e peroxidase no tratamento com FI, enquanto que, na SC foram lipoxigenase e AS. Depois da presença de M. oryzae a lipoxigenase e a fenilalanina-amônia liase apresentaram atividade tanto com FI quanto na SC, diferindo dos controles (plantas inoculadas com água e com M. oryzae, somente). S. oryzae apresentou variabilidade para as características avaliadas e potencial antagônico aos patógenos do arroz. As alterações na atividade enzimática indicam a indução de resistência em plantas na interação M. oryzae x arroz x S. oryzae.

Magnaporthe oryzae

Metabólito secundário

Biocontrole

Indução de risistência

Atividade enzimática

Magnaporthe oryzae

Secondary metabolite

Biocontrol

Induced resistance

Enzymatic activity

CIENCIAS AGRARIAS::AGRONOMIA

Bioprospecção de biomoléculas isoladas de fungos endofíticos de Combretum leprosum do bioma Caatinga / Bioprospection of biomolecule isolated from endophytic fungal of Combretum leprosum from Caatinga biome

Suikinai Nobre Santos

03 September 2012

Os micro-organismos que habitam o interior das plantas (endofíticos ou endófitos) tornaram-se foco de interesse por estarem envolvidos na produção de compostos químicos como enzimas, alcalóides, antibióticos, anticancerígenas e diferentes metabólitos. Os ecossistemas de regiões tropicais tem sido alvo de busca de compostos naturais por causa da riqueza de espécies e nichos ecológicos presentes nestas comunidades. O objetivo deste trabalho o isolamento, identificação e a bioprospecção de fungos endofíticos obtidos de Combretum leprosum e a detecção nos extratos de planta e micro-organismos da presença do composto combretastatin (CA4). Folhas, galhos, frutos e raízes de C. leprosum foram coletados de cinco estados dentro da zona de semiárido brasileiro: Bahia, Piauí, Ceará, Paraíba, Rio Grande do Norte. Partes das amostras foram triturados e submetidos à maceração primeiramente em diclorometano, seguidos de tetrahidrofurano e acetona de acordo com Pettit et al.(1987) para possível extração da CA4. Além disso, para avaliação in vitro da atividade citotóxica e antimicrobiana foram realizadas extrações em acetato de etila, clorofórmio e metanol. Foram detectados a possível presença da CA4 em todos os órgãos das plantas extraídos com tetrahidrofurano e as maiores concentrações foram observadas nas folhas. A atividade antitumoral dos extratos vegetais apresentaram as maiores inibições contra carcinoma (ovário IC50 10µg/mL-1, rim IC50 8,7µg/mL-1 e mama IC50 14,1µg/mL-1) e glioma.IC50 13,5µg/mL-1. A outra parte das amostras (folhas, caules e raízes) foram desinfetadas, fragmentadas e colocadas em meios de cultivo (Martin, BDA, Agar água) por 60 dias, 28°C. Foram isolados 405 fungos endofíticos e 159 apresentaram atividade contra fitopatogênicos, 72% para Rhizoctonia solani e 28% para Pythium aphanidermatum. As vinte e três linhagens que apresentaram as melhores atividades antifitopatogênicas foram submetidas a crescimento em Czapec em cultura estacionaria, por 30 dias, a 28°C, os respectivos metabólitos foram obtidos em múltiplo (3.0 e 11.0) e avaliados a atividade antimicrobiana contra bactérias patogênicas e fungos. Quatro linhagens foram selecionadas, identificadas pelo sequenciamento da região 18S, CFE177 como Fusarium oxysporum, CFE03 como Hypocrea koningii, linhagem CFE108 como Aspesgillus oryzae e CFE391 como Fusarium solani e avaliadas in vitro pelos testes biológicos: atividade antitumoral, antioxidante e antimicobactéria. Os compostos produzidos por A. oryzae CFE108 apresentaram potencial para bioprospecção, e de acordo com as atividade citotóxicas as maiores ações foram contra as linhagens linfoma histiocística (J744), mieloma murino (B16F10) e baixa citotóxidade para carcinoma de bexiga (ECV304) e leucemia eritroblástica humana (k562) na concentração de 1mg/mL-1. Foram isolados dois compostos: SS-XL-32-01 identificado como bis-(2-etilhexil) ftalato (DEHP) e SS-XL-20-1 identificado como fenol, 2.2 metilenobis[6-(1,1-dimetiletil)-4- etil], ambos com atividade anticâncer para células HeLa com percentual de ate 98% e 71%, de morte, respectivamente. Alem disso, a modificação através da reação de metilação do composto SS-XL-32-1 resultou na quebra do anel aromático, formação de 4 subprodutos e perda da atividade, sendo um indicativo do sitio ativo da molécula responsável pela atividade observada. Portanto, fungos endofíticos de 18 plantas do semiárido brasileiro podem ser considerados fonte de bioprospecção para novas moléculas bioativas com atividade antitumoral. / The micro-organisms that reside in the aerial tissues and roots of plants (endophytic or endophyte) became the focus of interest for being involved in the chemical production such as enzymes, alkaloids, antibiotics, anticancer and different metabolites. The ecosystems of tropical region have been targeted search of natural compounds because of the richness of species and ecological niches present in these communities. The aim of this work was the isolation, identification and bioprospection for endophytic fungi from Combretum leprosum and detection in extracts of the plant and micro-organisms for the presence of the combretastatin (CA4). Leaves, stems, fruits and roots of C. leprosum were collected from five states within the semi-arid zone of Brazil: Bahia, Piaui, Ceara, Paraiba, Rio Grande do Norte. Part of the samples were crushed and subjected to maceration in dichloromethane, followed by tetrahydrofuran and acetone according to Pettit et al. (1987) for extracting the possible CA4. Moreover, for in vitro evaluation of the cytotoxic and antimicrobial activity extractions were carried out in ethyl acetate, chloroform and methanol. Were detected the possible presence of CA4 all plant organs extracted with tetrahydrofuran and the highest concentrations were observed on the leaves. The antitumor activity of plant extracts showed the highest inhibition against carcinoma (ovary IC50 10µg/mL-1, kidney IC50 8.7 µg/mL-1 and breast IC50 14.1 µg/mL-1) glioma IC50 and 13.5 mg-/mL-1. The other part of the samples (leaves, stems and roots) were disinfected, fragmented and placed in culture media (Martin, PDA, water agar) for 60 days, 28°C. 405 Endophytic fungi were isolated and 159 showed activity against phytopathogenic, 72% for Rhizoctonia solani and 28% for Pythium aphanidermatum. Twenty-three strains that showed good activities antiphytopathogenic, were grow on medium Czapec in static culture, for 30 days at 28°C, the respective metabolites were obtained in multiples pH (3.0 and 11.0) and evaluated the antimicrobial activity against pathogenic bacteria and fungi. Four strains were selected, identified by sequencing the 18S region, CFE177 as Fusarium oxysporum, CFE03 as Hypocrea koningii, strain CFE108 as Aspesgillus oryzae and CFE391 Fusarium solani, and evaluated by in vitro biological tests: antitumor, antioxidant and antimicobactérium activity. The compounds produced by A. oryzae CFE108 had biological potential and in accordance with the cytotoxic activity, showed the highest activities against lymphoma lines (J744), murine myeloma (B16F10) and low cytotoxicity for carcinoma of the bladder (ECV304) and leukemia erythroblastic human (K562) in 1mg/mL-1 concentration. Two compounds were isolated: SS-XL-32- 01 identified as bis-(2-ethylhexyl)phthalate (DEHP), and SS-XL-20-1 as phenol 2.2methylenobis [6-(1,1-dimethylethyl) - 4-ethyl], both with anticancer activity for HeLa cells with a percentage of up to 98% and 71%, of death, respectively. In addition, modified by methylation reaction of the compound SS-XL-32-1 resulted in the breaking of the aromatic ring and result in formation of four product and loss of activity being indicative of the active site of the molecule can be the aromatic ring. Therefore, endophytic fungi in semiarid Brazil plant can be considered a source of bioprospection for new bioactive molecules with anticancer activity.

Aspergillus oryzae

Atividade antitumoral

Bioprospecção

Caatinga

Combretum leprosum

Metabólitos secundários

Micro-organismos endofíticos

Antitumor activity

Aspergillus oryzae

Bioprospection

Caatinga

Combretum leprosum

Endophytic fungi

Secondary metabolite

Semiarid

\"Produção de metabólitos antimicrobianos e sideróforos de isolados provenientes de Terra Preta Antropogênica da Amazônia Ocidental\" / Antimicrobial metabolites and siderophore produced by strains from Anthropogenic Dark Earth of the Occidental Amazon

Samanta Maria Gobbo Fedrizzi

30 November 2006

Os microrganismos atraem considerável atenção por serem uma fonte de compostos biotecnológicos e farmacêuticos. Diversos produtos naturais peptídicos produzidos por fungos e bactérias são sintetizados por grandes enzimas, conhecidas como peptídeo sintetase não ribossômica (NRPS) e policetídeo sintase (PKS). A bioprospecção dos microrganismos isolados do solo de Terra Preta Antropogênica (TPA) da Amazônia Ocidental é de grande importância para o conhecimento deste bioma tropical. Este estudo correlacionou a presença de sideróforos e de compostos antimicrobianos produzidos pelos microrganismos isolados de TPA e dos solos adjacentes com a presença dos genes que codificam para NRPS e PKS. Linhagens bacterianas foram isoladas das amostras do solo coletadas de 10, 20 e 40 cm de profundidade. Os isolados foram cultivados em meio líquido específico por 2 dias a 28oC. Um total de 143 isolados foi testado para a atividade de sideróforo e para isso, as linhagens foram inoculadas em um meio com baixa concentração de ferro (MM9) contendo o complexo cromoazurol S-Fe3. Do total, 72 isolados apresentaram reação positiva para a produção de sideróforo. O DNA genômico dos isolados foi extraído e a amplificação por PCR foi realizada usando iniciadores específicos para NRPS e PKS. Os resultados mostraram que quinze isolados apresentaram o gene que codifica para NRPS, vinte isolados para PKS e somente dez isolados apresentaram ambos os genes. A presença de genes de NRPS e PKS em 31% dos isolados testados sugere que a produção dos sideróforos possa ocorrer pela via não ribossomal. Dois isolados foram selecionados para estudos de identificação e caracterização dos compostos. O isolado TP11 foi identificado como Pseudomonas putida através de seqüenciamento do 16S rRNA e apresentou resultado negativo para hidroxamato e catecol, sugerindo que o tipo de sideróforo não possui nenhum destes grupos funcionais. O isolado TP16 foi identificado como Pseudomonas putida e apresentou produção de sideróforo do tipo catecol e hidroxamato, sugerindo a produção de mais de um sideróforo. Além disso, esta linhagem produziu um composto antimicrobiano, com atividade de sideróforo identificado por espectrometria de massas como pseudomonina com massa molar de 330 Da. / Microorganisms have attracted considerable attention as a source for biotechnological and pharmaceutical agents. Several peptidic natural products synthesized by fungi and bacteria are assembled by large enzymes, referred as nonribosomal peptide synthetase (NRPS) and polyketide synthase (PKS). Bioprospection of microorganisms isolated from Anthropological Dark Earth soil of Brazilian Occidental Amazon is of great importance to the knowledge of this tropical biome. This study aimed to correlate the presence of siderophores and antimicrobial compounds produced by microorganisms isolated from Dark Earth and adjacent soils of Brazilian Amazon with the presence of genes encoding NRPS and PKS. Bacterial strains were isolated from soil samples collected at 10, 20 and 40 cm depth. The isolates were grown in specific liquid medium for 2 d at 28oC. A total of 143 isolates were screened for siderophore activity and for this, bacterial strains were inoculated on plates containing an iron-limited medium (MM9) amended with a chromeazurol S-Fe3 complex. From the total, seventy-two isolates showed positive reaction for siderophore production. Genomic DNA of the isolates was extracted and PCR amplification was carried out using specific primers for NRPS and PKS. The results showed that fifteen isolates presented NRPS, twenty isolates presented PKS and only ten isolates showed both genes. The presence of NRPS and PKS genes in 31% of the isolates tested suggests that production of siderophores may occur by a nonribosomal pathway. Two isolates were selected for further studies. Isolate TP11 was identified as Pseudomonas putida by 16S rDNA sequencing analysis and was negative for hydroxamate and catechol, suggesting that the siderophore type has no hydroxamate- or catechol-type functional groups. The isolate TP16 was identified as Pseudomonas putida and showed the production of catechol and hydroxamate siderophore-type, suggesting the production of more than one siderophore. In addition, this strain produced an antimicrobial compound, with siderophore activity identified through mass spectrometry as pseudomonine with a molar mass of 330 Da.

16S rRNA

Metabólito Secundário

Peptídeo Sintetase Não Ribossômica

Policetídeo Sintase

Pseudomonina.

16S rRNA

Non-ribosomal Peptide Synthetase

Polyketide Synthase

Pseudomonine.

Secondary Metabolite

Caractérisation chimique des métabolomes secondaires de Penicillium et Fusarium par marquage isotopique couplé à la spectrométrie de masse haute résolution / Chemical caracterisation of the secondary metabolomes of penicillium and fusarium by isotope labelling and high resolution mass spectrometry

Hautbergue, Thaïs

14 November 2017

Une méthode permettant de caractériser l’ensemble du métabolome secondaire de moisissures a été appliquée à la caractérisation des métabolomes de Penicillium nordicum, Penicillium verrucosum et Fusarium graminearum. Le substrat représentant l’unique source de carbone et d’azote des moisissures, chacun des champignons ont été mis en culture sur trois types de grains de blé: (i) grains naturels, (ii) grains marqués à 97% de 13C, et (iii) grains marqués à 53% 13C et 97% de 15N. Les extraits ont été analysés par HRMS. Les métabolites secondaires ont été spécifiquement détectés et leurs formules brutes ont été caractérisées. La caractérisation de nouveaux métabolites secondaires a ensuite été assistées par la génération de réseaux moléculaires de similarités MS/MS. L’étude de P. verrucosum et P. nordicum a permis de détecter 98 et 92 métabolites secondaires respectivement. Parmi eux, 80% étaient inconnus. La génération de réseaux moléculaires a permis de mettre en évidence un groupe de 25 composés se fragmentant de manière similaire. Seize de ces composés ont été identifiés comme étant des dérivés de fungisporines, des métabolites suspectés d’intervenir dans la croissance aérienne des champignons. Des analyses structurales ont permis de caractériser de nouveaux composés potentiellement impliqués dans l’infestation des denrées alimentaires. Le marquage du métabolome de F. graminearum par des isotopes stables a permis de mettre en évidence la production de 37 métabolites secondaires dont 29 inconnus lorsque le champignon se développe in vitro. Des analyses par MSn ont permis d’élucider les structures des fusaristatines C et D. / Characterization of fungal secondary metabolomes became a great challenge in the last decades due to both the emergence of fungal threats, and the industrial interest of many natural products; In view of this, we recently developed an analytical strategy for fungal secondary metabolome characterization (Cano P. et al. Anal. Chem. (2013) 85:8412) based on untargeted MS metabolomics applied to labeled samples. This strategy has been here validated by application to the analysis of the complex secondary metabolomes of Penicillium verrucosum and Penicillium nordicum. HRMS acquisitions performed on specific isotopically labelled samples, MS/MS experiments and in-silico emerging tools such as molecular networks, allowed to characterize 181 metabolites, including 80% of new compounds, and the structural determination of seven potential new mycotoxins. Penicillium verrucosum (NRRL 5571) and Penicillium nordicum (NRRL 6062) were grown on wheat grains (Triticum aestivum) presenting different isotopic enrichments: (i) naturally enriched grains, (ii) 97% 13C, and (iii) 53% 13C / 97% 15N. Extracts of each culture were analyzed by HPLC coupled to a LTQ-Orbitrap mass spectrometer equipped with electrospray ionization, operating in the positive or the negative mode. Metabolites were then specifically detected according to the specific isotopic pattern of their respective isotopic enrichments. Known secondary metabolites were annotated using the Antibase database, then identified by comparison with standard compounds when available. Unknown secondary metabolites were annotated using molecular networks of MS/MS similarities (Watrous J. et al.; PNAS (2012) 109 E1743). Wheat grains representing the only source of carbon and nitrogen for fungal growth, the produced fungal secondary metabolites were either unlabeled (naturally enriched cultures), singly labeled (13C cultures) or doubly labeled (13C/15N cultures). This feature allowed discrimination of fungal metabolites against non-fungal compounds which remained unlabeled in the three substrates. Fungal origin was further confirmed by analysis of a control 12C wheat extract (without fungus). Furthermore, the comparison of m/z ratios of a same metabolite detected in the three different cultures, led to the unambiguous determination of the number of carbon and nitrogen atoms and therefore to the unambiguous characterization of its chemical formula. This approach previously developed and validated on a well characterized fungus, has been here successfully applied to the characterization of the complex and unknown secondary metabolomes of P. verrucosum and P. nordicum. Analyses of the two studied fungal strains allowed the detection of 181 secondary metabolites. Interestingly, only 20% of them are suspected to match known metabolites according to databases, meaning that 80% of this metabolome is unknown. To enhance unknown identification efficiency, a molecular network of MS/MS similarities has been generated from our data. A group of 24 metabolites with highly similar MS/MS spectra was highlighted on P. nordicum and P. verrucosum. Fifteen of them were identified as cyclic tetrapeptides from the fungisporin family. Tandem mass spectrometry experiments were performed to characterize the structure of these secondary metabolites. To the best of our knowledge, this is the first time these molecules are pointed out on these Penicillium species. More interestingly, seven of the other metabolites display some similarities with fungisporins, but have never been detected on fungal metabolomes. Furthermore, although the two studied strains are genetically close, these new metabolites seem to be strain specific.

Métabolome secondaire

Spectrométrie de masse

Penicillium

Fungisporine

Fusarium

Fusaristatine

Marquage isotopique

Réseaux moléculaires

Secondary metabolite

Mass spectrometry

Penicillium

Fungisporin

Fusarium

Fusaristatin

Isotope labeling

Molecular network

Développement technologique et bioproduction d’actifs pour la cosmétique à l'aide de cultures cellulaires végétales indifférenciées / Plant cell culture technology development and bioproduction for cosmetic

Guyon, Jean-Baptiste

17 December 2014

Les premières cultures cellulaires végétales in vitro ont été développées à partir de carotte, grâce à Gautheret en 1939. Il a obtenu ce résultat par la découverte au préalable du pouvoir de totipotence des cellules végétales (Haberland 1902). Afin d’obtenir les cellules indifférenciées Gautheret a utilisé des milieux de culture contenant des macroéléments (K, N et P), des microélements (Mg, B,…), des vitamines, du sucre et des phytohormones. Dans la littérature, plusieurs compositions sont souvent utilisées comme White (1934), Murashige and Skoog (1962)) ou Gamborg, Miller et Ojima (1970). Les nuances entre ces milieux se basent sur des concentrations modifiées en phosphates, nitrates ou en phytohormones (auxine/cytokinine). Chaque espèce a besoin d’un milieu particulier pour induire la callogénèse. En effet, selon l’origine (géographique) et le type d’explant (feuilles, racines, tiges,…) traité les conditions d’induction de la callogénèse varieront. De nombreuses personnes portent un intérêt aux cultures cellulaires pour leur utilisation en cosmétique ou en pharmacie. Actuellement, deux entreprises produisent ces cellules à l’échelle industrielle. Ainsi, Phyton Biotech (entreprise allemande) purifie du taxol à partir d’If (Taxus baccata) et Mitsui petrochemical produit de la skinonine à partir de grémils (Lithospernum erythrorizon). / The first plant cell culture has been developed by Gautheret in 1939 based on carrot plant cell tissus. He obtained these results through the discovery of the plant totipotency power (Haberland, 1902). He used for cal production a culture medium composed by macroelements (K, N, P…) and microelements (Mg, B …), vitamin, sugar. Later on, several mediums were used like and described in literature i.e. Murashige and Skoog (1962), White (1934) or Gamborg, Miller and Ojima (1970). The differences between such medium consisted mainly concentrations especially of phosphates, nitrates or auxin/cytokinine balance. However, each species needs specific medium for growth. Any people works of this subject and the interest for pharmaceutical and cosmetical industry grow up. Plant cell culture is a difficult technology an industrial use. Recently, two companies performed industrial production of taxol (Taxus baccata) and shikonin (Lithospernum erythrorizon) respectively PhytonBitotech and Mitsui petrochemical. My thesis work was to develop plant cell cultures fom unusual plants which can be used for the industrial production of cosmetics.

Culture in vitro végétale

Métabolites secondaires

Production industrielle

Biomasse

Phytohormones

Croissance

Bioréacteur

Cosmétique

Plant cell culture

Secondary metabolite

Industrial production

Biomass

Plant hormone

Growth

Bioreactor

Cosmetic