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  • About
  • The Global ETD Search service is a free service for researchers to find electronic theses and dissertations. This service is provided by the Networked Digital Library of Theses and Dissertations.
    Our metadata is collected from universities around the world. If you manage a university/consortium/country archive and want to be added, details can be found on the NDLTD website.
1

Utilization of Cellulosic Materials by Thermotoga petrophila

Chen, Li 06 November 2014 (has links)
Thermotoga petrophila is a hyperthermophilic anaerobic bacterium that grows optimally at 80?? C. It can utilize plant biomass to produce biofuels, including ethanol and hydrogen, which are alternative and renewable sources of energy. Xylan, microcrystalline avicel PH105, switchgrass, corn husks and wheat straw were used as growth substrates to determine T. petrophila???s capability to use different types of plant biomass for the production of ethanol and hydrogen. The metabolism of cellulosic substrates was analyzed by integrating proteomics analysis, gene identification, cellulase and xylanase activities, growth, metabolic products and cell adhesion. T. petrophila showed best growth on xylan, followed by corn husks, switchgrass, avicel PH105 and wheat straw. The optimal pH for higher biofuel yield was within the range of 8.0 to 8.5. The metabolic end products were H2, CO2, acetate, lactate, formate and succinate when T. petrophila grew on all the tested cellulosic materials. The highest yield of hydrogen (9.6 mM) and the highest yield of ethanol (0.95 mM) were both detected when T. petrophila was grown on xylan. No growth was observed on xylose, which was not expected because T. petrophila grew very well on xylan, a ??-1, 4-xylopryranose polymer from which xylose can be produced upon hydrolysis. The possible reason for this phenomenon may be that T. petrophila has no specific sugar transporters for xylose, although it contains all the genes encoding xylose metabolizing enzymes. The majority of exoglucanases and endoglucanases presented in T. petrophila were extracellular enzymes. The highest specific activities of exoglucanase (1361.3 mU/mg) and endoglucanase (1032.1 mU/mg) in T. petrophila were found in the supernatants of the growth culture with xylan as the sole substrate, indicating that xylan, not cellulose, is the best inducer to increase the expression of extracellular cellulases. Compared to the huge discrepancy of extracellular cellulases activities among different substrates (from 0 to 1361.3 mU/mg), intracellular cellulase (endoglucanase) activity was relatively steady (around 150 mU/mg). Xylanase activity was also detected in both the supernatant and the cell free extract; thus T. petrophila contains both extracellular and intracellular xylanase. The highest xylanase activity was detected in the cell free extract when T. petrophila was grown on cellobiose and xylan (3732.4 mU/mg and 3152.8 mU/mg, respectively), indicating that the majority of xylanase is an intracellular enzyme, and xylan and cellobiose are the best inducers to increase the expression of xylanase. Adhesion of T. petrophila cells to xylan, with many filaments connecting all the cells, was observed using scanning electron microscope and fluorescent staining microscope, whereas there was no attachment between cells and cellulose. This difference may explain why T. petrophila grew much better on xylan than on cellulose because cell adhesion increases enzyme concentration near the substrate to improve the efficiency of cellulosic material utilization. Furthermore, proteomics analysis was used to quantify all the expressed proteins in different growth media with various substrates. The proteomics data revealed that the most important enzymes for cellulose and hemicellulose utilization were ATP binding cassette (ABC) transporters, S-layer proteins and membrane binding proteins, which were up-regulated when T. petrophila was grown on cellulosic materials. The sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) also indicated the up-regulated proteins from the media with cellulosic substrates were probably ABC transporters and S-layer proteins based on the size of proteins. Based on the gene identification, end product determination and proteomics analysis, the tentative cellulosic material metabolic pathways in T. petrophila were completely profiled. Overall, our results suggest that the ability of T. petrophila to convert cellulosic materials into hydrogen and ethanol exceeds T. maritima, which is a model strain for studying hyperthermophiles. T. petrophila has great potential in applications of producing highly thermostable cellulases and biofuels from cellulosic materials. However, the mechanism of cell adhesion between T. petrophila and xylan and the regulation of the entire cellulosic materials metabolic pathway need further investigation.
2

Estudos da estabilidade, flexibilidade e atividade enzimática da B-mananase da bactéria hipertermofílica Thermotoga petrophila

Silva, Viviam Moura da January 2014 (has links)
Orientador: Prof. Dr. Wanius José Garcia da Silva / Dissertação (mestrado) - Universidade Federal do ABC, Programa de Pós-Graduação em Biotecnociência, 2014. / A proteina endo-B-1,4-mananase da bacteria Thermotoga petrophila (TpMan) e uma enzima hipertermoestavel que catalisa a hidrolise de ligacoes B-1,4-manosidicas em varios polissacarideos contendo manana. Um recente estudo mostrou que a enzima TpMan e composta de um dominio catalitico GH5 e um dominio de ligacao ao carboidrato CBM27 conectados atraves de um linker, entretanto, ate o momento, a estrutura tridimensional cristalografica nao foi determinada para a enzima completa. Pouco se sabe sobre a conformacao da enzima TpMan intacta como tambem o papel do comprimento e flexibilidade do linker sobre o arranjo espacial dos dominio constitutivos. Neste estudo, nos reportamos a primeira caracterizacao estrutural da enzima TpMan completa utilizando a tecnica de espalhamento de raios-X a baixos angulos (SAXS) combinada com a estrutura tridimensional dos dominios individuais para elucidar o modelo de baixa resolucao, as dimensoes globais, e a flexibilidade desta enzima modular em diferentes temperaturas. Nossos resultados sao consistentes com um linker que apresenta uma estrutura compacta e que ocupa um pequeno volume quando comparado com seu grande numero de residuos de aminoacidos (102 residuos de aminoacidos). Alem disso, a 20 oC os resultados sao consistentes com um modelo onde a enzima TpMan e um monomero composto de tres dominios e que apresenta nivel de flexibilidade molecular em solucao. Mesmo a enzima intacta apresentando algum grau de flexibilidade, existe uma conformacao preferivel, a qual pode ser descrita pelo procedimento de modelagem de corpo rigido. Finalmente, os resultados indicam que a enzima TpMan sofre uma transicao dependente da temperatura entre estados conformacionais de sua estrutura secundaria regular. Nossos resultados sugerem que o linker pode otimizar a geometria entre os outros dois dominios com respeito ao substrato a altas temperaturas. Os estudos apresentados aqui devem proporcionar uma base util para futuros estudos biofisicos da enzima TpMan intacta.

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