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31	Comunidade microbiana e produção de metano em reator anaeróbio em batelada com metilamina como fonte de carbono / Microbial community and methane production in anaerobic batch reactor with methylamine as carbon source Vich, Daniele Vital 13 August 2010 (has links) A degradação da metilamina foi investigada por meio da avaliação da velocidade específica máxima de produção de metano (VEM CH4) e da comunidade microbiana relacionada aos Domínios Bacteria e Archaea. Para isso, foram realizados dois ensaios com reatores anaeróbios em batelada inoculados com lodo granulado oriundo de reator UASB usado no tratamento de água residuária de abatedouro de aves. Em todos os ensaios, os reatores controle, que não receberam adição de metilamina, apresentaram VEM CH4 de 0,04 mmol/L g STV dia. O primeiro ensaio avaliou a degradação da metilamina em diferentes concentrações de inóculo (2,5, 5,0 e 10,0 g STV/L) e substrato (1.550 e 3.100 mg metilamina/L). A concentração de \'CH IND.4\' esperada estequiometricamente foi atingida em todos os reatores (37,50 e 75,00 mmol \'CH IND.4\'/L, para concentrações de 1.550 e 3.100 mg metilamina/L, respectivamente), exceto para aquele com 2,5 g STV/L e 3.100 mg metilamina/L, que produziu somente 2,04 mmol \'CH IND.4\'/L. A maior velocidade específica máxima de produção de \'CH IND.4\' foi 4,42 mmol/L g STV dia, obtida nos reatores com 2,5 g STV/L e 1.550 mg metilamina/L. Os reatores inoculados com 5,0 g STV/L tiveram VEM CH4 de 2,31 e 2,34 para 1.550 e 3.100 mg metilamina/L, respectivamente. Os reatores com 1.550 mg metilamina/L e 10,0 g STV/L apresentaram VEM CH4 de 1,28 mmol/L g STV dia. A concentração de \'N\'-\'NH IND.4\'POT.+\' excedeu em 12,9%, 0,7% e 18,3% o valor esperado (698 mg/L) para os reatores com 1.550 mg metilamina/L e 2,5, 5,0 e 10,0 g STV/L, respectivamente. Nos reatores com 3.100 mg metilamina/L, as concentrações finais de \'N\'-\'NH IND.4\'POT.+\' foram 122 e 1.726 mg/L para concentrações de inóculo de 2,5 e 5,0 g STV/L, respectivamente. O segundo ensaio comparou diferentes relações metilamina/sulfato (0,71, 1,26 e 2,18) em reatores inoculados com 5,0 g STV/L contendo 1.550 mg metilamina/L. As concentrações de \'CH IND.4\' esperadas estequiometricamente foram atingidas em todos os reatores. As velocidades específicas máximas de formação de \'CH IND.4\' foram de 2,54, 2,31 e 3,14 mmol/L g STV dia para as relações metilamina/sulfato 0,71, 1,26 e 2,18, respectivamente. Em todos os reatores, a concentração de \'N\'-\'NH IND.4\'POT.+\' atingiu média final de 1200 mg/L. Os reatores controle consumiram 71,9% do sulfato adicionado. Os reatores com relação metilamina/sulfato 0,71, 1,26 e 2,18 consumiram 49,6%, 61,6% e 83,2% de todo o sulfato adicionado, respectivamente. Nos dois ensaios, os exames microscópicos revelaram a presença de cocos, bacilos, filamentos, cocos e sarcinas fluorescentes. Nos reatores alimentados apenas com metilamina, o seqüenciamento de fragmentos da região 16S do RNAr detectou cinco Filos do Domínio Bacteria (Acidobacteria 4%, Firmicutes 11%, Proteobacteria 14%, Spirochaetes 13% e Synergistes 47%). Nos reatores com metilamina e sulfato, sete Filos foram detectados (Firmicutes 45%, Proteobacteria 7%, Spirochaetes 2%, Synergistes 16%, Chloroflexi 4%, Thermotogae 8% e Planctomycetes 1%). Nos dois ensaios, o Domínio Archaea foi predominantemente representado pelas Famílias Methanomicrobiaceae, Methanosaetaceae e Methanosarcinaceae, com presença de Methanomethylovorans hollandica, uma espécie de arquéia metanogênica com metabolismo especializado na degradação de metilamina. / The degradation of methylamine was investigated assessing the maximum specific methane production rate (MSR CH4) and the microbial community related to Bacteria e Archaea Domains. For this, two tests were performed in anaerobic batch reactors inoculated with granular sludge from an UASB reactor used in the treatment of poultry wastes. In all experiments, the control reactors, without methylamine addition, showed MSR CH4 of 0.04 mmol/L g TVS day. The first experiment evaluated the degradation of methylamine at different inoculum concentrations (2.5, 5.0 and 10.0 g TVS/L) and substrate concentrations (1,550 and 3,100 mg methylamine/L). The stoichiometrically expected \'CH IND.4\' concentration was reached in all reactors (37.50 and 75.00 mmol \'CH IND.4\'/L, for methylamine concentrations of 1,550 and 3,100 mg methylamine/L, respectively), except for the reactor with 2.5 g TVS/L and 3,100 mg methylamine/L, that produced only 2.04 mmol \'CH IND.4\'/L. The highest maximum specific methane production rate was 4.42 mmol/L g TVS day, reached in the reactors with 2.5 g TVS/L and 1,550 mg methylamine/L. The reactors inoculated with 5.0 g TVS/L had MSR CH4 of 2.31 and 2.34 for 1,550 and 3,100 mg methylamine/L, respectively. The reactors with 1,550 mg methylamine/L and 10.0 g TVS/L had MSR CH4 of 1.28 mmol/L g TVS day. The \'N\'-\'NH IND.4\'POT.-\' concentrations exceeded 12.9%, 0.7% and 18.3% the expected value (698 mg/L) for the reactors with 1,550 mg methylamine/L and 2.5, 5.0 and 10.0 g TVS/L, respectively. In the reactors with 3,100 mg methylamine/L, the final concentrations of \'NH IND.4\'POT.+\'-\'N\' were 122 and 1,726 mg/L for inoculum concentrations of 2.5 and 5.0 g TVS/L, respectively. The second experiment compared different methylamine/sulfate ratios (0.71, 1.26 and 2.18) on reactors inoculated with 5.0 g TVS/L containing 1,550 mg methylamine/L. The stoichiometrically expected \'CH IND.4\' concentration was reached in all reactors. The maximum specific methane production rates were 2.54, 2.31 and 3.14 mmol/L g TVS day for methylamine/sulfate ratios of 0.71, 1.26 and 2.18, respectively. In all reactors, the average \'NH IND.4\'POT.+\'-\'N\' final concentration was 1,200 mg/L. The control reactors consumed 71.9% of the added substrate. The reactors with methylamine/sulfate ratios of 0.71, 1.26 and 2.18 consumed 49.6%, 61.6% and 83.2% of all the added sulfate, respectively. In both experiments, the microscopic analysis revealed cocci, rods, filaments, fluorescent cocci and sarcinas. In the reactors fed with methylamine only, the sequencing of 16S rRNA fragments detected five Phyla of the Bacteria Domain (Acidobacteria 4%, Firmicutes 11%, Proteobacteria 14%, Spirochaetes 13% and Synergistes 47%). In the reactors with methylamine and sulfate, seven Phyla were detected (Firmicutes 45%, Proteobacteria 7%, Spirochaetes 2%, Synergistes 16%, Chloroflexi 4%, Thermotogae 8% e Planctomycetes 1%). In both experiments, Archaea Domain was mainly represented by Methanomicrobiaceae, Methanosaetaceae and Methanosarcinaceae Families, with the presence of Methanomethylovorans hollandica, a methanogenic archaea specie with specific metabolism for methylamine degradation. Anaerobic biological treatment Arquéias metanogênicas Metanogênese Methanogenesis Methanogenic archaea Methanomethylovorans Methanomethylovorans Methylamine Metilamina Redução de sulfato Sulfate reduction Tratamento biológico anaeróbio
32	Influência do oxigênio no crescimento de arquéias metanogênicas e bactérias redutoras de sulfato em reatores anaeróbios em batelada / Oxygen influence on methanogenic archaea and sulfate reducing bacteria\'s growth in anaerobic batch reactors Sarti, Érika Lamaro 10 May 2007 (has links) Este trabalho teve como objetivo avaliar o comportamento de arquéias metanogênicas e bactérias redutoras de sulfato na presença de oxigênio, em reatores anaeróbios em batelada, sob condições sulfetogênicas e mesofílicas. Os reatores foram inoculados com lodo anaeróbio proveniente de reator UASB utilizado no tratamento de água residuária de avicultura. Triplicatas de reatores foram alimentadas com meio basal ZINDER, acrescido de acetato de sódio, etanol ou lactato de sódio e sulfato de sódio, de modo a se obter relações DQO/sulfato iniciais de 1,1-1,5. O headspace dos reatores foi preenchido com \'N IND.2\' (100%) acrescido de oxigênio puro comercial (3-3,5 mg/L de oxigênio dissolvido). Os reatores anaeróbios controle foram alimentados com os mesmos substratos orgânicos, entretanto, seu headspace foi preenchido com \'N IND.2\'/\'CO IND.2\' (70/30%). Nos reatores com acetato de sódio, etanol e lactato de sódio as velocidades de produção de metano foram de 0,30 mmol/L.h, 0,41 mmol/L.h e 0,16 mmol/L.h, respectivamente, para os reatores controle. Em relação aos reatores com oxigênio os valores foram de 0,27 mmol/L.h, 0,40 mmol/L.h e 0,08 mmol/L.h, respectivamente. Na presença de acetato, etanol e lactato a redução de sulfato foi de 57% e 97%; 59,6% e 76,6%; 77,5% e 41,9%, respectivamente, nos reatores controle e com oxigênio. Nos reatores com acetato e etanol houve predomínio de organismos do domínio Archaea nos reatores controle (59,2% e 58,8%) e com oxigênio (60,7% e 54,5%), respectivamente. No reator controle contendo lactato, também ocorreu o predomínio de arquéias metanogênicas (56,2%), enquanto na presença de oxigênio houve predomínio de organismos do domínio Bacteria (63,9%). As proporções de BRS nos reatores controle e com oxigênio contendo acetato, etanol e lactato foram de 22% e 17,3%; 28% e 16,9%; 19,5% e 21,9%, respectivamente. O oxigênio não inibiu a metanogênese e nem a redução de sulfato nos reatores contendo acetato e etanol. / This work aimed to evaluate the behavior of methanogenic archaea and sulfate reducing bacteria in the presence of oxygen, using anaerobic batch reactors under sulfidogenic and mesophilic conditions. The reactors were inoculated with anaerobic sludge from UASB reactor treating poultry wastes. Third copies of the reactors were fed with ZINDER medium, increased with sodium acetate, ethanol or sodium lactate and sodium sulfate, in order to get COD/sulfate ratio of 1,1-1,5. The headspace of the reactors was filled with \'N IND.2\' (100%) and increased with oxygen (OD concentration of 3-3.5 mg/L). The anaerobic control reactors were fed with the same organics substrates, however, the headspace was filled with \'N IND.2\'/\'CO IND.2\' (70/30%). The rates of methane production were 0.30 mmol/L.h, 0.41 mmol/L.h and 0.16 mmol/L.h, in acetate, ethanol and lactate controls reactors, respectively. In oxygen reactors, the rates of methane production were 0.27 mmol/L.h, 0.40 mmol/L.h and 0.08 mmol/L.h in acetate, ethanol and lactate reactors, respectively. The rates of sulfate reduction in acetate, ethanol and lactate reactors were 57% and 97%; 59.6% and 76.6%; 77.5% and 41.9%, respectively, in control reactors and oxygen reactors. In acetate and ethanol reactors, were verified predominance of Archaea domain in control reactors (59.2% and 58.8%) and oxygen reactors (60.7% and 54.5%), respectively. In lactate control reactor also was verified predominance of Archaea domain (56.2%), whereas in lactate oxygen reactors there was predominance of cells belonging to Bacteria domain (63.9%). BRS ratio in acetate, ethanol and lactate control reactors and oxygen reactors corresponded to 22% and 17.3%; 28% and 16.9%; 19.5% and 21.9%, respectively. The addition of oxygen didn\'t inhibit the methanogenesis and sulfate reduction in acetate reactors and in ethanol reactors. Arquéias metanogênicas Bactérias redutoras de sulfato Batch reactors and FISH FISH Methanogenic archaeas Oxigênio Oxygen Reatores em batelada Sulfate reducing bacteria
33	Digestão anaeróbia de dejeitos suínos: um estudo para verificar a influência da adição de meios de cultura. / Anaerobic digestion of swine litter: a study to verify the influence of the addition of culture media. GOMES, Damião Junior. 28 May 2018 (has links) Submitted by Deyse Queiroz (deysequeirozz@hotmail.com) on 2018-05-28T14:27:42Z No. of bitstreams: 1 DAMIÃO JUNIOR GOMES - DISSERTAÇÃO PPGSA PROFISSIONAL 2014..pdf: 1021631 bytes, checksum: 9d3b509edbbf52efa1db00de496731a6 (MD5) / Made available in DSpace on 2018-05-28T14:27:42Z (GMT). No. of bitstreams: 1 DAMIÃO JUNIOR GOMES - DISSERTAÇÃO PPGSA PROFISSIONAL 2014..pdf: 1021631 bytes, checksum: 9d3b509edbbf52efa1db00de496731a6 (MD5) Previous issue date: 2014-12-19 / Este estudo analisa o comportamento físico químico e microbiológico, referente à mistura de resíduos suínos com e sem adição de meios de cultura descartados, durante o processo de biodigestão anaeróbia, em biorreator tipo batelada. Montaram-se dois biorreatores, para fim de comparação, com capacidade de 50L cada. Os biorreatores foram ativados com a mesma diluição, razão de 1:2 (mistura biomassa/água, em m/m), no entanto, em um deles foi acrescidos 10% (m/m) de meios de culturas usados oriundos de um laboratório microbiológico. O monitoramento destes procedera por 56 dias, sendo coletadas alíquotas dos substratos nos tempos 0, 7, 21, 28, 35, 42, 49 e 56 dias, e submetidos à caracterização físico-química e microbiológica, bem como, verificou-se a influência dos meios de cultura na produção de biogás. Durante o desenvolvimento não se realizou nenhuma suplementação nos biodigestores. Os dados experimentais apontaram que durante o processo da biodegradação anaeróbia dos substratos, o biorreator A (com presença de meios de cultura) desempenhou melhores resultados, em relação ao biorreator B (com ausência de meios de cultura). Como por exemplo, pH’s próximos da alcalinidade, propiciando o desenvolvimento das bactérias metanogênicas, e consequentemente, maior liberação de gases. No que concerne aos valores de concentração de coliformes totais (35 ºC), termotolerantes (45 ºC) e E. coli entre os afluentes e efluentes dos biorreatores, estes foram reduzidos, principalmente no biodigestor A, em que apresentou maior concentração de macronutrientes (NPK). Por fim, pode ser inferido que os resultados foram bastante relevantes, fazendo entender que a introdução de meios de cultura potencializa as reações de biodigestão anaeróbia, favorecendo maior produção de biogás, além de incorporar ao efluente (biofertilizante) maior concentração de nutrientes. / This study analyzes the chemical and physical behavior microbiological, regarding the mixture of swine residues with and without addition of discarded culture means, during the process of anaerobic digestion, in bioreactor boat-load type. Two bioreactors were set up, for comparison end, with capacity of 50L each. The bioreactors were activated with the same dilution, reason of 1 : 2 (it mixes biomass / water, in m/m), however , in one of them was added 10 % (m/m) of means of cultures used originating from of the microbiological laboratory . The monitoring of these it had proceeded for 56 days , being collected brackets of the substrata in the times 0, 7, 21, 28 , 35, 42, 49 and 56 days, and submitted to the physiochemical characterization and microbiological, as well as, the influence of the culture means was verified in the biogas production. During the development it did not take place any supplementation in the digesters. The trial date appeared that during the process of the anaerobic biodegradation of the substrates, the bioreactor (with presence of culture means) it carried October better results, in relation to the bioreactor B (with absence of culture means). For example, close pH 's of the alkalinity , propitiating the development of the methanogenic bacteria , and consequently , larger liberation of gases. In what it concerns to the values of concentration of the total coliforms (35 ° C), thermophilic (45 ° C) and E. coli between the tributaries and effluents of the bioreactors, these were reduced, mainly in the digester, in that It presented larger macronutrient concentration (NPK ). Finally, it can be inferred which the results were quite relevant, making that to understand the introduction of culture means potentiates the reactions of anaerobic digestion , favoring larger biogas production, fouled Incorporating to the effluent (biofertilizer) larger concentration of nutritious. Biodigestão anaeróbia. Produção de biogás. Bactérias metanogênicas. Macronutrientes. Biofertilizante. Dejetos suínos. Anaerobic Biodigestion. Biogas production. Methanogenic bacteria. Macronutrients. Biofertilizer. Swine manure.
34	Influência do oxigênio no crescimento de arquéias metanogênicas e bactérias redutoras de sulfato em reatores anaeróbios em batelada / Oxygen influence on methanogenic archaea and sulfate reducing bacteria\'s growth in anaerobic batch reactors Érika Lamaro Sarti 10 May 2007 (has links) Este trabalho teve como objetivo avaliar o comportamento de arquéias metanogênicas e bactérias redutoras de sulfato na presença de oxigênio, em reatores anaeróbios em batelada, sob condições sulfetogênicas e mesofílicas. Os reatores foram inoculados com lodo anaeróbio proveniente de reator UASB utilizado no tratamento de água residuária de avicultura. Triplicatas de reatores foram alimentadas com meio basal ZINDER, acrescido de acetato de sódio, etanol ou lactato de sódio e sulfato de sódio, de modo a se obter relações DQO/sulfato iniciais de 1,1-1,5. O headspace dos reatores foi preenchido com \'N IND.2\' (100%) acrescido de oxigênio puro comercial (3-3,5 mg/L de oxigênio dissolvido). Os reatores anaeróbios controle foram alimentados com os mesmos substratos orgânicos, entretanto, seu headspace foi preenchido com \'N IND.2\'/\'CO IND.2\' (70/30%). Nos reatores com acetato de sódio, etanol e lactato de sódio as velocidades de produção de metano foram de 0,30 mmol/L.h, 0,41 mmol/L.h e 0,16 mmol/L.h, respectivamente, para os reatores controle. Em relação aos reatores com oxigênio os valores foram de 0,27 mmol/L.h, 0,40 mmol/L.h e 0,08 mmol/L.h, respectivamente. Na presença de acetato, etanol e lactato a redução de sulfato foi de 57% e 97%; 59,6% e 76,6%; 77,5% e 41,9%, respectivamente, nos reatores controle e com oxigênio. Nos reatores com acetato e etanol houve predomínio de organismos do domínio Archaea nos reatores controle (59,2% e 58,8%) e com oxigênio (60,7% e 54,5%), respectivamente. No reator controle contendo lactato, também ocorreu o predomínio de arquéias metanogênicas (56,2%), enquanto na presença de oxigênio houve predomínio de organismos do domínio Bacteria (63,9%). As proporções de BRS nos reatores controle e com oxigênio contendo acetato, etanol e lactato foram de 22% e 17,3%; 28% e 16,9%; 19,5% e 21,9%, respectivamente. O oxigênio não inibiu a metanogênese e nem a redução de sulfato nos reatores contendo acetato e etanol. / This work aimed to evaluate the behavior of methanogenic archaea and sulfate reducing bacteria in the presence of oxygen, using anaerobic batch reactors under sulfidogenic and mesophilic conditions. The reactors were inoculated with anaerobic sludge from UASB reactor treating poultry wastes. Third copies of the reactors were fed with ZINDER medium, increased with sodium acetate, ethanol or sodium lactate and sodium sulfate, in order to get COD/sulfate ratio of 1,1-1,5. The headspace of the reactors was filled with \'N IND.2\' (100%) and increased with oxygen (OD concentration of 3-3.5 mg/L). The anaerobic control reactors were fed with the same organics substrates, however, the headspace was filled with \'N IND.2\'/\'CO IND.2\' (70/30%). The rates of methane production were 0.30 mmol/L.h, 0.41 mmol/L.h and 0.16 mmol/L.h, in acetate, ethanol and lactate controls reactors, respectively. In oxygen reactors, the rates of methane production were 0.27 mmol/L.h, 0.40 mmol/L.h and 0.08 mmol/L.h in acetate, ethanol and lactate reactors, respectively. The rates of sulfate reduction in acetate, ethanol and lactate reactors were 57% and 97%; 59.6% and 76.6%; 77.5% and 41.9%, respectively, in control reactors and oxygen reactors. In acetate and ethanol reactors, were verified predominance of Archaea domain in control reactors (59.2% and 58.8%) and oxygen reactors (60.7% and 54.5%), respectively. In lactate control reactor also was verified predominance of Archaea domain (56.2%), whereas in lactate oxygen reactors there was predominance of cells belonging to Bacteria domain (63.9%). BRS ratio in acetate, ethanol and lactate control reactors and oxygen reactors corresponded to 22% and 17.3%; 28% and 16.9%; 19.5% and 21.9%, respectively. The addition of oxygen didn\'t inhibit the methanogenesis and sulfate reduction in acetate reactors and in ethanol reactors. Arquéias metanogênicas Bactérias redutoras de sulfato FISH Oxigênio Reatores em batelada Batch reactors and FISH Methanogenic archaeas Oxygen Sulfate reducing bacteria
35	Comunidade microbiana e produção de metano em reator anaeróbio em batelada com metilamina como fonte de carbono / Microbial community and methane production in anaerobic batch reactor with methylamine as carbon source Daniele Vital Vich 13 August 2010 (has links) A degradação da metilamina foi investigada por meio da avaliação da velocidade específica máxima de produção de metano (VEM CH4) e da comunidade microbiana relacionada aos Domínios Bacteria e Archaea. Para isso, foram realizados dois ensaios com reatores anaeróbios em batelada inoculados com lodo granulado oriundo de reator UASB usado no tratamento de água residuária de abatedouro de aves. Em todos os ensaios, os reatores controle, que não receberam adição de metilamina, apresentaram VEM CH4 de 0,04 mmol/L g STV dia. O primeiro ensaio avaliou a degradação da metilamina em diferentes concentrações de inóculo (2,5, 5,0 e 10,0 g STV/L) e substrato (1.550 e 3.100 mg metilamina/L). A concentração de \'CH IND.4\' esperada estequiometricamente foi atingida em todos os reatores (37,50 e 75,00 mmol \'CH IND.4\'/L, para concentrações de 1.550 e 3.100 mg metilamina/L, respectivamente), exceto para aquele com 2,5 g STV/L e 3.100 mg metilamina/L, que produziu somente 2,04 mmol \'CH IND.4\'/L. A maior velocidade específica máxima de produção de \'CH IND.4\' foi 4,42 mmol/L g STV dia, obtida nos reatores com 2,5 g STV/L e 1.550 mg metilamina/L. Os reatores inoculados com 5,0 g STV/L tiveram VEM CH4 de 2,31 e 2,34 para 1.550 e 3.100 mg metilamina/L, respectivamente. Os reatores com 1.550 mg metilamina/L e 10,0 g STV/L apresentaram VEM CH4 de 1,28 mmol/L g STV dia. A concentração de \'N\'-\'NH IND.4\'POT.+\' excedeu em 12,9%, 0,7% e 18,3% o valor esperado (698 mg/L) para os reatores com 1.550 mg metilamina/L e 2,5, 5,0 e 10,0 g STV/L, respectivamente. Nos reatores com 3.100 mg metilamina/L, as concentrações finais de \'N\'-\'NH IND.4\'POT.+\' foram 122 e 1.726 mg/L para concentrações de inóculo de 2,5 e 5,0 g STV/L, respectivamente. O segundo ensaio comparou diferentes relações metilamina/sulfato (0,71, 1,26 e 2,18) em reatores inoculados com 5,0 g STV/L contendo 1.550 mg metilamina/L. As concentrações de \'CH IND.4\' esperadas estequiometricamente foram atingidas em todos os reatores. As velocidades específicas máximas de formação de \'CH IND.4\' foram de 2,54, 2,31 e 3,14 mmol/L g STV dia para as relações metilamina/sulfato 0,71, 1,26 e 2,18, respectivamente. Em todos os reatores, a concentração de \'N\'-\'NH IND.4\'POT.+\' atingiu média final de 1200 mg/L. Os reatores controle consumiram 71,9% do sulfato adicionado. Os reatores com relação metilamina/sulfato 0,71, 1,26 e 2,18 consumiram 49,6%, 61,6% e 83,2% de todo o sulfato adicionado, respectivamente. Nos dois ensaios, os exames microscópicos revelaram a presença de cocos, bacilos, filamentos, cocos e sarcinas fluorescentes. Nos reatores alimentados apenas com metilamina, o seqüenciamento de fragmentos da região 16S do RNAr detectou cinco Filos do Domínio Bacteria (Acidobacteria 4%, Firmicutes 11%, Proteobacteria 14%, Spirochaetes 13% e Synergistes 47%). Nos reatores com metilamina e sulfato, sete Filos foram detectados (Firmicutes 45%, Proteobacteria 7%, Spirochaetes 2%, Synergistes 16%, Chloroflexi 4%, Thermotogae 8% e Planctomycetes 1%). Nos dois ensaios, o Domínio Archaea foi predominantemente representado pelas Famílias Methanomicrobiaceae, Methanosaetaceae e Methanosarcinaceae, com presença de Methanomethylovorans hollandica, uma espécie de arquéia metanogênica com metabolismo especializado na degradação de metilamina. / The degradation of methylamine was investigated assessing the maximum specific methane production rate (MSR CH4) and the microbial community related to Bacteria e Archaea Domains. For this, two tests were performed in anaerobic batch reactors inoculated with granular sludge from an UASB reactor used in the treatment of poultry wastes. In all experiments, the control reactors, without methylamine addition, showed MSR CH4 of 0.04 mmol/L g TVS day. The first experiment evaluated the degradation of methylamine at different inoculum concentrations (2.5, 5.0 and 10.0 g TVS/L) and substrate concentrations (1,550 and 3,100 mg methylamine/L). The stoichiometrically expected \'CH IND.4\' concentration was reached in all reactors (37.50 and 75.00 mmol \'CH IND.4\'/L, for methylamine concentrations of 1,550 and 3,100 mg methylamine/L, respectively), except for the reactor with 2.5 g TVS/L and 3,100 mg methylamine/L, that produced only 2.04 mmol \'CH IND.4\'/L. The highest maximum specific methane production rate was 4.42 mmol/L g TVS day, reached in the reactors with 2.5 g TVS/L and 1,550 mg methylamine/L. The reactors inoculated with 5.0 g TVS/L had MSR CH4 of 2.31 and 2.34 for 1,550 and 3,100 mg methylamine/L, respectively. The reactors with 1,550 mg methylamine/L and 10.0 g TVS/L had MSR CH4 of 1.28 mmol/L g TVS day. The \'N\'-\'NH IND.4\'POT.-\' concentrations exceeded 12.9%, 0.7% and 18.3% the expected value (698 mg/L) for the reactors with 1,550 mg methylamine/L and 2.5, 5.0 and 10.0 g TVS/L, respectively. In the reactors with 3,100 mg methylamine/L, the final concentrations of \'NH IND.4\'POT.+\'-\'N\' were 122 and 1,726 mg/L for inoculum concentrations of 2.5 and 5.0 g TVS/L, respectively. The second experiment compared different methylamine/sulfate ratios (0.71, 1.26 and 2.18) on reactors inoculated with 5.0 g TVS/L containing 1,550 mg methylamine/L. The stoichiometrically expected \'CH IND.4\' concentration was reached in all reactors. The maximum specific methane production rates were 2.54, 2.31 and 3.14 mmol/L g TVS day for methylamine/sulfate ratios of 0.71, 1.26 and 2.18, respectively. In all reactors, the average \'NH IND.4\'POT.+\'-\'N\' final concentration was 1,200 mg/L. The control reactors consumed 71.9% of the added substrate. The reactors with methylamine/sulfate ratios of 0.71, 1.26 and 2.18 consumed 49.6%, 61.6% and 83.2% of all the added sulfate, respectively. In both experiments, the microscopic analysis revealed cocci, rods, filaments, fluorescent cocci and sarcinas. In the reactors fed with methylamine only, the sequencing of 16S rRNA fragments detected five Phyla of the Bacteria Domain (Acidobacteria 4%, Firmicutes 11%, Proteobacteria 14%, Spirochaetes 13% and Synergistes 47%). In the reactors with methylamine and sulfate, seven Phyla were detected (Firmicutes 45%, Proteobacteria 7%, Spirochaetes 2%, Synergistes 16%, Chloroflexi 4%, Thermotogae 8% e Planctomycetes 1%). In both experiments, Archaea Domain was mainly represented by Methanomicrobiaceae, Methanosaetaceae and Methanosarcinaceae Families, with the presence of Methanomethylovorans hollandica, a methanogenic archaea specie with specific metabolism for methylamine degradation. Arquéias metanogênicas Metanogênese Methanomethylovorans Metilamina Redução de sulfato Tratamento biológico anaeróbio Anaerobic biological treatment Methanogenesis Methanogenic archaea Methanomethylovorans Methylamine Sulfate reduction
36	Avaliação da comunidade microbiana anaeróbia em reator sulfetogênico utilizando a hibridação in situ com sondas fluorescentes (FISH) / Evaluation of anaerobic microbial community in sulfidogenic reactor using fluorescent in situ hybridization (FISH) Hirasawa, Julia Sumiko 25 April 2003 (has links) Neste trabalho foi realizada a caracterização microbiana anaeróbia de reatores anaeróbios diferenciais horizontais e em batelada, operados sob condições sulfetogênicas e mesofílicas (30ºC). Os reatores diferenciais foram preenchidos com diferentes materiais suportes (espuma de poliuretano, carvão vegetal, polietileno reciclado de baixa densidade e cerâmica porosa à base de alumina) visando a seleção do suporte adequado para otimização do processo sulfetogênico, para a relação DQO/sulfato de aproximadamente 0,67. Os reatores diferenciais foram alimentados diariamente com esgoto sintético, contendo aproximadamente 1000 mg/L de DQO e 1500 mg/L de sulfato, durante 28 dias de operação. A caracterização microbiana foi realizada através da técnica de hibridação in situ fluorescente (FISH), microscopia óptica e eletrônica de varredura. Foram realizadas quantificações, em termos de porcentagens, de microrganismos pertencentes ao Domínio Bacteria (EUB338), Domínio Archaea (ARC915) e bactérias redutoras do íon sulfato (BRS) da subdivisão delta de Proteobacteria (SRB385). Nos reatores diferenciais, houve predomínio de bactérias em todos os suportes estudados. Os reatores diferenciais operados com espuma e carvão apresentaram maiores porcentagens de BRS, com valores iguais a 57,6% e 69,7%, respectivamente. A cerâmica foi o material que apresentou melhor equilíbrio de bactérias e arqueas metanogênicas, com 59,6% e 40,9%, respectivamente. Os reatores em batelada foram operados com espuma de poliuretano e carvão vegetal com relação DQO/sulfato de aproximadamente 3. As porcentagens de BRS quantificadas pelo FISH foram iguais a 65,3% e 69,1% para espuma e carvão, respectivamente. Em ambos os reatores o carvão vegetal foi o material mais favorável à sulfetogênese. / This research reports an anaerobic microbial characterization of both, a horizontal differential anaerobic and a batch reactors, operated at sulfidogenic and mesofilic conditions at 30ºC. The differential reactors were filled with four support materials (polyurethane foam, vegetable coal, recycled polyethylene of low density and alumin based porous ceramic) aiming the selection of a more appropriated support for optimization of sulfidogenic processes (ratio COD/sulfate of approximately 0.67). Differential reactors were fed daily with synthetic sewage, containing approximately 1000 mg/L of COD and 1500 mg/L of sulfate concentrations, during 28 days of operation. Microbial characterization was accomplished using fluorescent in situ hybridization (FISH), optic and scanning electronic microscopy. It was realized a quantification, in percentages, of microorganisms belong to Bacteria Domain (EUB338), Archaea Domain (ARC915) and sulfate-reducing bacteria (SRB) of delta subdivision Proteobacteria (SRB385). Differential reactors have shown predominance of bacteria in all the support materials studied. Differential reactors operated with foam and coal presented the greatest percentages of SRB, with values equal to 57.6% and 69.7%, respectively. The ceramic was the material that presented the best equilibrium of bacteria and methanogenic archaea, with 59.6% and 40.9%, respectively. Batch reactors were operated with polyurethane foam and vegetable coal with COD/sulfate ratio of approximately 3. Percentages of SRB quantified by FISH were equals to 65.3% and 69.1% for foam and coal, respectively. In both reactors the vegetable coal have shown to be the most favorable material to sulfidogenesis. Arqueas metanogênicas Bactérias redutoras de sulfato FISH FISH Material suporte Methanogenic archaea Sulfate-reducing bacteria Sulfetogênese Sulfidogenesis Support material
37	Etude de microbiote digestif africain par culturomics et nouvelle technique d'isolement et de culture de Methanobrevibacter smithii / African digestive microbiote studies by culturomics and a new studies culturomics and a new technique of isolation and culture of Methanobrevibacter smithii Traore, Sory Ibrahima 23 November 2018 (has links) L’étude du microbiote digestif a connu un regain d’intérêt au début des années 2000, avec l’avènement des techniques moléculaires. La culturomics a démontré sa complémentarité depuis 2010 en réduisant une partie des biais des méthodes moléculaires. Une revue sur les techniques d’étude du microbiote digestif et l’analyse du microbiote des sujets africains. Les études de métagénomique en Afrique ont révélé une augmentation de la biodiversité, en particulier des Spirochaetes et des Prevotella chez les africains par rapport aux occidentaux. Sur les 1162 bactéries isolées par culturomics, 476 n'étaient pas africaines, 445 étaient communes et 241 étaient d’origine africaine dont 68 nouvelles espèces. Pour ma participation au travail de culturomics, 102750 colonies testées par MALDI-TOF,ont permis d'identifier 377 espèces incluant 40 nouvelles espèces,17 nouveaux genres et 2 nouvelles familles.Ces nouvelles espèces ont été décrites par taxonogenomics ou new species announcement.Les archaea méthanogènes ont une prévalence de 97,4% pour M. smithii et associés à des pathologies comme l’abcès du cerveau,les parodontites etc. La culture est fastidieuse et nécessitait une source extérieure d’hydrogène. Sous enceinte anaérobie, nous avons cultivé avec succès M. smithii à partir d’un milieu de culture liquide inoculé d’échantillon de selle. L’isolement en culture pure a été un succès sur milieu gélosé en réalisant une coculture avec Bacteroides thetaiotaomicron. Nous avons aussi testé avec succès la coculture de M. smithii avec d’autres bactéries productrices d’hydrogène connues. Les tests de chromatographie en phase gazeuse montraient que ces souches produisaient de l’hydrogène. / The study of the digestive microbiota was a renewed interest in the early 2000s, with the advent of molecular techniques. The culturomics has demonstrated its complementarity since 2010 by reducing some of the biases of molecular methods. A review on the techniques of studying the digestive microbiota and the analysis of the microbiota of African subjects. Metagenomic studies in Africa have revealed an increase in biodiversity, especially Spirochaetes and Prevotella among Africans compared to Westerners. Of the 1162 bacteria isolated by culturomics, 476 were non-African, 445 were common, and 241 were of African origin, including 68 new species. For my participation in the work of culturomics, 102750 colonies tested by MALDI-TOF, identified 377 species including 40 new species, 17 new genera and 2 new families. These new species have been described by taxonogenomics or new species announcement.Methanogenic archaea have a prevalence of 97.4% for M. smithii and associated with pathologies such as brain abscess, periodontitis and so on. The cultivation is tedious and required an external source of hydrogen. Under anaerobic enclosure, we successfully cultivated M. smithii from a liquid culture medium inoculated with a stool sample. The isolation in pure culture was a success on agar medium by performing a coculture with Bacteroides thetaiotaomicron. We have also successfully tested the co-culture of M. smithii with other known hydrogen-producing bacteria. Gas chromatographic tests showed that these strains produced hydrogen. Microbiote humain Microbiote africain Microbial culturomics Archaea méthanogènes Methanobrevibacter smithii Human microbiota African microbiota Microbial culturomics Methanogenic Archaea Methanobrevibacter smithii
38	Methanogens from Siberian permafrost as models for life on Mars : response to simulated martian conditions and biosignature characterization Serrano, Paloma January 2014 (has links) Mars is one of the best candidates among planetary bodies for supporting life. The presence of water in the form of ice and atmospheric vapour together with the availability of biogenic elements and energy are indicators of the possibility of hosting life as we know it. The occurrence of permanently frozen ground – permafrost, is a common phenomenon on Mars and it shows multiple morphological analogies with terrestrial permafrost. Despite the extreme inhospitable conditions, highly diverse microbial communities inhabit terrestrial permafrost in large numbers. Among these are methanogenic archaea, which are anaerobic chemotrophic microorganisms that meet many of the metabolic and physiological requirements for survival on the martian subsurface. Moreover, methanogens from Siberian permafrost are extremely resistant against different types of physiological stresses as well as simulated martian thermo-physical and subsurface conditions, making them promising model organisms for potential life on Mars. The main aims of this investigation are to assess the survival of methanogenic archaea under Mars conditions, focusing on methanogens from Siberian permafrost, and to characterize their biosignatures by means of Raman spectroscopy, a powerful technology for microbial identification that will be used in the ExoMars mission. For this purpose, methanogens from Siberian permafrost and non-permafrost habitats were subjected to simulated martian desiccation by exposure to an ultra-low subfreezing temperature (-80ºC) and to Mars regolith (S-MRS and P-MRS) and atmospheric analogues. They were also exposed to different concentrations of perchlorate, a strong oxidant found in martian soils. Moreover, the biosignatures of methanogens were characterized at the single-cell level using confocal Raman microspectroscopy (CRM). The results showed survival and methane production in all methanogenic strains under simulated martian desiccation. After exposure to subfreezing temperatures, Siberian permafrost strains had a faster metabolic recovery, whereas the membranes of non-permafrost methanogens remained intact to a greater extent. The strain Methanosarcina soligelidi SMA-21 from Siberian permafrost showed significantly higher methane production rates than all other strains after the exposure to martian soil and atmospheric analogues, and all strains survived the presence of perchlorate at the concentration on Mars. Furthermore, CRM analyses revealed remarkable differences in the overall chemical composition of permafrost and non-permafrost strains of methanogens, regardless of their phylogenetic relationship. The convergence of the chemical composition in non-sister permafrost strains may be the consequence of adaptations to the environment, and could explain their greater resistance compared to the non-permafrost strains. As part of this study, Raman spectroscopy was evaluated as an analytical technique for remote detection of methanogens embedded in a mineral matrix. This thesis contributes to the understanding of the survival limits of methanogenic archaea under simulated martian conditions to further assess the hypothetical existence of life similar to methanogens on the martian subsurface. In addition, the overall chemical composition of methanogens was characterized for the first time by means of confocal Raman microspectroscopy, with potential implications for astrobiological research. / Der Mars ist unter allen Planeten derjenige, der aufgrund verschiedener Faktoren am wahrscheinlichsten Leben ermöglichen kann. Das Vorhandensein von Wasser in Form von Eis und atmosphärischem Dampf zusammen mit der Verfügbarkeit biogener Elemente sowie Energie sind Indikatoren für die Möglichkeit, Leben, wie wir es kennen, zu beherbergen. Das Auftreten von dauerhaft gefrorenen Böden, oder auch Permafrost, ist ein verbreitetes Phänomen auf dem Mars. Dabei zeigen sich vielfältige morphologische Analogien zum terrestrischen Permafrost. Permafrostgebiete auf der Erde, welche trotz extremer, Bedingungen durch eine große Zahl und Vielfalt mikrobieller Gemeinschaften besiedelt sind, sind hinsichtlich möglicher Habitate auf dem Mars die vielversprechendste Analogie. Die meisten methanogenen Archaeen sind anaerobe, chemolithotrophe Mikroorganismen, die auf der Marsoberfläche viele der metabolischen und physiologischen Erfordernisse zum Überleben vorfinden. Methanogene Archaeen aus dem sibirischen Permafrost sind zudem extrem resistent gegenüber unterschiedlichen Formen von physiologischem Stress sowie simulierten thermo-physikalischen Marsbedingungen. Die Hauptziele dieser Untersuchung bestehen darin, das Überleben der methanogenen Archaeen unter Marsbedingungen zu beurteilen, wobei der Fokus auf methanogenen Archaeen aus dem sibirischen Permafrost liegt, sowie deren Biosignaturen mit Hilfe der Raman-Spektroskopie zu charakterisieren, einer starken Technologie zur mikrobiellen Identifikation, welche bei der ExoMars-Mission zum Einsatz kommen wird. Zu diesem Zweck wurden methanogene Archaeen aus dem sibirischen Permafrost sowie aus Nicht-Permafrost-Habitaten in Simulationen Marsbedingungen ausgesetzt, wie Austrocknung durch Langzeitversuche bei ultraniedrigen Temperaturen unter dem Gefrierpunkt (-80ºC), Mars-analogen Mineralien (S-MRS und P-MRS) sowie einer Marsatmosphäre. Weiterhin wurden die Kulturen verschiedenen Konzentrationen von Magnesiumperchlorat, einem starken Oxidant, der im Marsboden nachgewiesenen wurde, ausgesetzt. Ferner wurden die Biosignaturen einzelner Zellen der methanogenen Archaeen mit Hilfe der konfokalen Raman-Mikrospektroskopie (CRM) charakterisiert. Die Ergebnisse zeigten für alle untersuchten methanogenen Stämme Überleben und Methanbildung, nachdem diese simulierten Austrocknungsbedingungen ausgesetzt worden waren. Nach Versuchen mit Temperaturen unter dem Gefrierpunkt zeigten die Stämme aus dem sibirischen Permafrost eine schnellere Wiederaufnahme der Stoffwechseltätigkeit, wohingegen bei den Referenzorganismen aus Nicht-Permafrost-Habitaten die Zell¬membranen im größeren Ausmaß intakt blieben. Der Stamm Methanosarcina soligelidi SMA-21 aus dem sibirischen Permafrost zeigte nach dem Belastungstest mit Marsboden und Mars-analoger Atmosphäre signifikant höhere Methanbildungsraten. Zudem überlebten alle untersuchten Stämme die Zugabe von Magnesiumperchlorat in der entsprechenden Konzentration, die auf dem Mars vorkommt. Weiterhin konnten durch die Raman-Spektroskopie beachtliche Unterschiede in der chemischen Zusammensetzung zwischen methanogenen Archaeen aus Permafrost- und Nicht-Permafrost-Habitaten, trotz ihrer phylogenetischen Verwandtschaft, ermittelt werden. Die Konvergenz der chemischen Zusammensetzung der Permafrost-Stämme könnte das Resultat ihrer Anpassung an die Umgebung sein, was auch die Unterschiede hinsichtlich ihrer Resistenz verglichen mit Nicht-Permafrost-Stämmen erklären könnte. Als Teil dieser Studie wurde die Raman-Spektroskopie als Analyse-Technik zur Ferndetektion von methanogenen Archaeen, welche in eine Mineral-Matrix eingebettet sind, evaluiert. Diese Dissertation trägt zu einem besseren Verständnis hinsichtlich der Grenzen für ein Überleben von methanogenen Archaeen unter simulierten Marsbedingungen bei und damit zu einer Beurteilung der Hypothese, ob es ähnliches Leben unter der Marsoberfläche geben könnte. Darüber hinaus wurde erstmalig die chemische Zusammensetzung von methanogenen Archaeen mit Hilfe der Raman-Mikrospektroskopie charakterisiert. Dieser Technologie kommt eine wesentliche Bedeutung für weitere Forschungstätigkeit in der Astrobiologie zu. Mars Raman Spektroskopie Biosignaturen methanogenic archaea Siberian permafrost Mars Raman spectroscopy biosignatures Life sciences
39	Desempenho de sistema composto por reatores anaeróbios em série seguido de filtro biológico percolador no tratamento de águas residuárias de suinocultura Duda, Rose Maria [UNESP] 24 February 2010 (has links) (PDF) Made available in DSpace on 2014-06-11T19:32:54Z (GMT). No. of bitstreams: 0 Previous issue date: 2010-02-24Bitstream added on 2014-06-13T20:24:21Z : No. of bitstreams: 1 duda_rm_dr_jabo.pdf: 7705565 bytes, checksum: 22edf4cc4e57fedc9fa2426e83e181e0 (MD5) / Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP) / Avaliou-se o desempenho de um reator anaeróbio de fluxo ascendente com manta de lodo (UASB) seguido de um filtro anaeróbio de fluxo ascendente, instalados em série, com volume total de 300 L e 190 L, respectivamente, no tratamento de águas residuárias de suinocultura. As cargas orgânicas volumétricas aplicadas no reator UASB foram de 9,2 a 26,7 g DQOtotal (L d)-1. Para o pós-tratamento do efluente do sistema de tratamento anaeróbio utilizou-se um filtro biológico percolador (FBP) com volume total de 250 L. O meio suporte utilizado no filtro anaeróbio e no FBP foi composto por anéis de bambu e anéis de eletroduto plástico corrugado. As cargas hidráulicas superficiais (Qs) aplicadas no FBP variaram de 3,5 a 21,1 m3 (m2 d)-1. Os tempos de detenção hidráulica (TDH) aplicados no sistema de tratamento anaeróbio e pós-tratamento foram de 23,3 a 66,6 h. As produções volumétricas de metano no sistema de tratamento anaeróbio variaram de 0,16 a 0,68 L CH4 (L reator d)-1. Foram observadas eficiências médias de remoção de até 97% para a demanda química de oxigênio total, de 98% para os sólidos suspensos totais, de 78% para o nitrogênio total, de 79% para o fósforo total, de 99,9% para o cobre, de 99,9% para o zinco e de 99,99% para os coliformes termotolerantes, no sistema de tratamento anaeróbio e póstratamento. Com a utilização de diferentes fontes de substrato no ensaio de atividade da microbiota, observou-se o crescimento equilibrado das populações hidrolíticas, acidogênicas, acetogênicas e metanogênicas acetoclásticas e hidrogenotróficas no lodo dos reatores anaeróbios. Com a aplicação da técnica de biologia molecular (metagenômica) foram identificadas no lodo do reator UASB e do filtro anaeróbio de fluxo ascendente arquéias metanogênicas das famílias Methanomicrobiaceae, Methanobacteriacea, Methanosaetaceae e Methanosarcinaceae. / The performance of an upflow anaerobic sludge blanket (UASB) followed of the anaerobic filter, installed in series, were evaluated for the treatment of swine wastewater. The total volume of UASB and anaerobic filter were of 300 L and 190 L, respectively. The organic load rate applied on the reactor UASB were of 9.2 to 26.7 g total COD (L d)-1, in the start and assays 1, 2, 3 and 4. For the post-treatment of effluent the anaerobic system was used a trickling filter, with total volume of 250 L. The supports used in the anaerobic filter and trickling filter were composed by bamboo rings in the start up and assays 1 to 2 and plastics rings in the assays 3 to 4. The hydraulic load applied on the trickling filter were of 3.5 to 21.1 m3 (m2 d)-1. The hydraulic detetion time (HDT) applied of system anaerobic and post treatment were 23.3 at 66.6 h. The volumetric methane productions ranged from 0.16 a 0.68 L CH4 (L reactor d)-1. The efficiencies of removal the chemical oxygen demand, total solids suspended, copper, zinc and fecal coliforms were of up to 97, 98, 78, 79, 99.9, 99.9 e 99.99%, respectively, for the anaerobic and post-treatment. With the use of different substratum sources in the assays of specific methanogenic activity, it was observed the balanced growth of the populations of microorganisms in the sludge of anaerobic reactor. The archaeas of the families Methanomicrobiaceae, Methanobacteriaceae; Methanosaetaceae and Methanosarcinaceae were identified in the sludge of the reactor UASB and of the anaerobic filter. Aguas residuais Atividade metanogênica Arquéias metanogênicas Carga orgânica volumétrica Specific methanogenic activity Organic load rate Anaerobic digestion Nutrients Post-treatment
40	Využití fugátu při pěstování kukuřice na siláž / Use of fugatami in the cultivation of corn silage VESELÁ, Miluše January 2015 (has links) The operation of biogas plants solves environmental aspects (energy management, reduction of negative impacts on the environment, use of renewable energy sources) and their influence in connection with the production of acidogenic (solid) as well as methanogenic (liquid) digestate. This requires establishing mandatory solution procedures in terms of the current legislation (air protection, use of fertilizers). The research for the thesis was carried out in the Agricultural and Commercial Cooperative in Kámen (in the region of Havlíčkův Brod), which lies 527 metres above the sea level. A biogas station has been operated by the cooperative since 2011. In addition to biogas, the cooperative also utilizes the fermentation remnants separated methanogenic digestate as a fertilizer and acidogenic digestate as a raw material for the production of compost. The thesis examined the use of methanogenic digestate when growing silage maize. During the one-year research, two maize hybrids and their response to fertilization by methanogenic digestate were assessed. Both hybrids achieved a higher yield of biomass and a higher yield of the dry matter.

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