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Microbial communities in organic substrates used for oil sands reclamation and their link to boreal seedling growthBeasse, Mark L Unknown Date
No description available.
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Active heterotrophic microbial communities from polar desert soils of the Canadian High ArcticTaghavimehr,Elham Unknown Date
No description available.
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15N stable isotope probing of pulp and paper wastewatersAddison, Sarah Louise January 2008 (has links)
Stable isotope probing (SIP) is an established technique that can be applied to identify the metabolically active micro-organisms within a microbial population. The SIP method utilises an isotopically-labelled substrate and PCR techniques to discern the members of a microbial community that incorporate the isotope into their DNA or RNA. The current literature gap around using 15N isotopes with RNA-SIP offers real potential and advantages for targeting and identifying active members from mixed communities involved in global biogeochemical nitrogen cycling. This study specifically investigated whether nitrogen based compounds can be used as substrates in RNA-SIP methodologies and whether they can in turn be used to probe mixed community environments known to be actively fixing nitrogen. The nitrogen-limited systems targeted represented an ideal opportunity to assess the suitability of 15N-RNA-SIP approaches due to their known high nitrogen fixation rates. Identifying these nitrogen-fixing bacteria could provide a better representation analysis of the community, leading to an improved prediction on how to manage and optimise the treatment performance of target waste systems and to exploit the unique bioconversion properties of these types of organisms. Initially, the project undertook methodological proof of concept by using a soluble nitrogen source, 15NH4Cl, to label the RNA of Novosphingobium nitrogenifigens and a mixed microbial community. Successful separation of the 14N- (control) and 15N-RNA was achieved for both pure and mixed communities using isopycnic caesium trifluoroacetate (CsTFA) gradients in an ultracentrifuge. The usefulness of this technique to identify active diazotrophs in real environmental samples was tested using a nitrogen-fixing community from a pulp and paper wastewater treatment system. After growing the mixed culture with 15N2 as the sole nitrogen source, the labelled RNA was extracted and fractionated using isopycnic centrifugation in CsTFA gradients. The community composition of the active nitrogen-fixing community in the 15N2 enriched fraction was analysed by establishing a 16S rRNA gene clone library containing over 200 members. These were analysed by comparison with published sequences and by phylogenetic analysis. It was found that the more isotopic label substrate incorporated, the further the buoyant density (BD) separation between 15N- and 14N-RNA. Novosphingobium nitrogenifigens gave an average BD shift of 0.03 + 0.004 g ml-1 (95.0 atom % 15N) with 15NH4Cl. For mixed communities the average BD shift was 0.02 + 0.004 g ml-1 (80.0 atom % 15N) with 15NH4Cl and 0.013 + 0.002 g ml-1 (32.6 atom % 15N) when using 15N2. Clone library analysis of 16S rRNA genes present in the enriched 15N-RNA fraction of the mixed community was shown to consist of a diverse population of bacteria as indicated by a Shannon Weaver index value of gt;2.8. Three dominant genera (Aeromonas, Pseudomonas and Bacillus) were identified by comparison with published sequences and phylogenetic analysis. Many other groups not known as archetypal nitrogen-fixing bacteria were also identified, demonstrating that 15N2-RNA-SIP provides a useful tool for the identification of important and previously unknown contributors to nitrogen fixation in a range of environments. Overall, this project has established that nitrogen based RNA-SIP is a powerful tool that can be used successfully and reproducibly with both pure and complex mixed microbial communities to study active diazotrophs in environmental samples.
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Characterization of Active Cellulolytic Consortia from Arctic TundraDunford, Eric Andrew January 2011 (has links)
The consortia of microorganisms responsible for the hydrolysis of cellulose in situ are at present poorly characterized. Nonetheless, the importance of these communities is underscored by their capacity for converting biomass to greenhouse gases such as carbon dioxide and methane. The metabolic capacities of these organisms is particularly alarming considering the volume of biomass that is projected to re-enter the carbon cycle in Arctic tundra soil environments as a result of a warming climate. Novel cold-adapted cellulase enzymes also present enormous opportunities for a broad range of industries. DNA stable-isotope probing (DNA-SIP) is a powerful tool for linking the phylogenetic identity and function of cellulolytic microorganisms by the incorporation of isotopically labelled substrate into nucleic acids. By providing 13C-enriched glucose and cellulose to soil microcosms, it was possible to characterize the communities of microorganisms involved in the metabolism of these substrates in an Arctic tundra soil sample from Resolute Bay, Canada. A protocol for generating 13C-enriched cellulose was developed as part of this thesis, and a visual DNA-SIP protocol was generated to demonstrate the experimental outline. Denaturing gradient gel electrophoresis (DGGE) and 16S rRNA clone libraries were used to visualize changes in community structure and to identify prevalent, active phylotypes in the SIP incubations. Notably, predominant phylotypes changed over time and clustered based on substrate metabolism. Labelled nucleic acids identified by sequenced DGGE bands and 16S rRNA gene clone libraries provided converging evidence indicating the predominance of Clostridium and Sporolactobacillus in the 13C-glucose microcosms, and Betaproteobacteria, Bacteroidetes, and Gammaproteobacteria in the 13C-cellulose microcosms. Active populations consuming glucose and cellulose were distinct based on principle coordinate analysis of “light” and “heavy” DNA. A large portion of the recovered sequences possessed no close matches in the GenBank database, reflecting the paucity of data on these communities of microorganisms.
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Active methane oxidizing bacteria in a boreal peat bog ecosystemEsson, Kaitlin Colleen 12 January 2015 (has links)
Boreal peatlands are important ecosystems to the global carbon cycle. Although they cover only 3% of the earth's land surface area, boreal peatlands store roughly one third of the world's soil carbon. Peatlands also comprise a large natural source of methane emitted to the atmosphere. Some methane in peatlands is oxidized before escaping to the atmosphere by aerobic methane oxidizing bacteria. With changing climate conditions, the fate of the stored carbon and emitted methane from these systems is uncertain. One important step toward better understanding the effects of climate change on carbon cycling in peatlands is to ascertain the microorganisms actively involved in carbon cycling. To investigate the active aerobic methane oxidizing bacteria in a boreal peat bog, a combination of microcosm experiments, DNA-stable isotope probing, and next generation sequencing technologies were employed. Studies were conducted on samples from the S1 peat bog in the Marcell Experimental Forest (MEF). Potential rates of methane oxidation were determined to be in the range of 13.85 to 17.26 μmol CH₄ g dwt⁻¹ d⁻¹. After incubating with ¹³C-CH₄, DNA was extracted from these samples, separated into heavy and light fractions with cesium chloride gradient formation by ultracentrifugation and needle fractionation, and fractions were fingerprinted with automated ribosomal intergenic spacer analysis (ARISA) and further interrogated with qPCR. Based on ARISA, distinct banding patterns were observed in heavy fractions in comparison to the light fractions indicating an incorporation of ¹³C into the DNA of active methane oxidizers. This was further supported by a relative enrichment in the functional gene pmoA, which encodes a subunit of the particulate methane monooxygenase, in heavy fractions from samples incubated for fourteen days. Within heavy fractions for samples incubated for 8 and 14 days, the relative abundance of methanotrophs increased to 37% and 25%, respectively, from an in situ abundance of approximately 4%. Phylogenetic analysis revealed that the methanotrophic community was composed of both Alpha and Gammaproteobacterial methanotrophs of the genera Methylocystis, Methylomonas, and Methylovulum. Both Methylocystis and Methylomonas have been detected in peatlands before, however, none of the phylotypes in this study were closely related to any known cultivated members of these groups. These data are the first to implicate Methylovulum as an active methane oxidizer in peatlands, though this organism has been detected in another cold aquatic ecosystem with consistent methane emissions. The Methylovulum sequences from this study, like Methylocystis and Methylomonas, were not closely related to the only cultivated member of this genus. While Methylocystis was dominant in ¹³C-enriched fractions with a relative abundance of 30% of the microbial community after an eight-day incubation, Methylomonas became dominant with a relative abundance of approximately 16% after fourteen days of incubation. The relative abundance of Methylovulum was maintained at 2% in ¹³C- enriched fractions after eight and fourteen days.
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Characterization of Active Cellulolytic Consortia from Arctic TundraDunford, Eric Andrew January 2011 (has links)
The consortia of microorganisms responsible for the hydrolysis of cellulose in situ are at present poorly characterized. Nonetheless, the importance of these communities is underscored by their capacity for converting biomass to greenhouse gases such as carbon dioxide and methane. The metabolic capacities of these organisms is particularly alarming considering the volume of biomass that is projected to re-enter the carbon cycle in Arctic tundra soil environments as a result of a warming climate. Novel cold-adapted cellulase enzymes also present enormous opportunities for a broad range of industries. DNA stable-isotope probing (DNA-SIP) is a powerful tool for linking the phylogenetic identity and function of cellulolytic microorganisms by the incorporation of isotopically labelled substrate into nucleic acids. By providing 13C-enriched glucose and cellulose to soil microcosms, it was possible to characterize the communities of microorganisms involved in the metabolism of these substrates in an Arctic tundra soil sample from Resolute Bay, Canada. A protocol for generating 13C-enriched cellulose was developed as part of this thesis, and a visual DNA-SIP protocol was generated to demonstrate the experimental outline. Denaturing gradient gel electrophoresis (DGGE) and 16S rRNA clone libraries were used to visualize changes in community structure and to identify prevalent, active phylotypes in the SIP incubations. Notably, predominant phylotypes changed over time and clustered based on substrate metabolism. Labelled nucleic acids identified by sequenced DGGE bands and 16S rRNA gene clone libraries provided converging evidence indicating the predominance of Clostridium and Sporolactobacillus in the 13C-glucose microcosms, and Betaproteobacteria, Bacteroidetes, and Gammaproteobacteria in the 13C-cellulose microcosms. Active populations consuming glucose and cellulose were distinct based on principle coordinate analysis of “light” and “heavy” DNA. A large portion of the recovered sequences possessed no close matches in the GenBank database, reflecting the paucity of data on these communities of microorganisms.
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Studying the Temporal Dynamics of the Gut Microbiota Using Metabolic Stable Isotope Labeling and MetaproteomicsSmyth, Patrick 29 June 2021 (has links)
The gut microbiome and its metabolic processes are dynamic systems. Surprisingly, our understanding of gut microbiome dynamics is limited. Here we report a metaproteomic workflow that involves protein stable isotope probing (protein-SIP) and identification/quantification of partially labeled peptides. We also developed a package, which we call MetaProfiler, that corrects for false identifications and performs phylogenetic and time series analysis for the study of microbiome dynamics. From the stool sample of five mice that were fed with 15-N hydrolysate from Ralstonia eutropha, we identified 15,297 non-redundant unlabeled peptides of which 10,839 of their heavy counterparts were quantified. These peptides revealed incorporation profiles over time that were different between and within taxa, as well as between and within clusters of orthologous groups (COGs). Our study helps unravel the complex dynamics of protein synthesis and bacterial dynamics in the mouse gut microbiome.
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Resource Legacies and Priming Regulate Microbial Communities in Antarctica's Dry ValleysSaurey, Sabrina Deni 07 June 2013 (has links) (PDF)
Multiple mechanisms control bacterial community structure but two in particular, the "legacy" of past environmental conditions, and the "priming" of bacteria to respond to seasonal or reoccurring fluctuations in resources, have the potential to determine both bacterial communities, as well as, temporal shifts in active bacterial taxa. To begin to evaluate the legacy effects of resources on microbial communities, we added four limiting resources annually (i.e., water only; C-mannitol + water; N-NH4NO3 + water; and C, N + water) and measured shifts in bacterial community composition after seven years in a cold desert ecosystem in the McMurdo Dry Valleys, Antarctica. Further, to investigate the ecological significance of priming, we conducted a series of stable isotope probing experiments (i.e., 18O-DNA SIP with 18O-labeled water, 13C-DNA SIP with 13C-labeled mannitol, 15N-DNA with 15N- NH4NO3, and a combined C and N SIP) and characterized the responding (i.e., isotopically labeled) and seed bank (i.e., unlabeled) bacterial communities. We performed each of the SIPs in soil microcosms corresponding to a single resource manipulation (e.g., 13C-labeled mannitol in C addition soils). We hypothesized that all long-term additions of nutrients and water will lead to a distinct bacterial community—a legacy effect due to the nutrient and water impoverished state of Antarctica soils. We also hypothesized that the stronger the legacy effects demonstrated by a specific community the more adapted or primed bacterial species will be to take advantage of the resource and respond. As hypothesized, resource additions created distinct bacterial legacy but to different degrees among the treatments. The extent of the resource legacy effects was greatest in the CN, intermediate in water and N, and lowest in C communities relative to the control communities, suggesting that C induced changes in communities were intensified by tandem N additions and that water alone created a more distinct legacy than water and C additions combined. Contrary to our hypothesis, the stronger the legacy effects, the less adapted or primed the community was to take advantage of resource additions. For example, the CN treatment that induced the greatest effect on bacterial communities had the lowest number of species (20.9%) in common between the responding and seed bank communities. This inverse relationship may be due to only two species (i.e., Arthrobacter, Actinobacteria and Massilia, Betaproteobacteria) really being primed to take advantage of CN and these species constituting over 75% of the seed bank community. Water, N, and C additions had similar levels of priming with 38.4%, 41.4%, and 36.3% of the responding species being present in the seed bank community, respectively. But of these three treatments, only the priming with water resulted in a unique responding community, suggesting that water, a universal bacterial resource, was enough to prime bacteria. Furthermore, water generates the most diverse responding community of all the resources with stemming from all of the fourteen dominant phyla. We did find patterns of ecological coherence among the responders, especially in the major responders (i.e., responders that increased in relative recovery by at least ten-fold). These responders were predominantly found in only three phyla (i.e., Actinobacteria, Bacteriodetes, and Gammaproteobacteria) regardless of resource addition. Alternatively minor responders (i.e., responders that increased in relative recovery at least two-fold) were contained in fourteen different phyla with specific taxa stimulated by CN (i.e., Betaproteobacteria) and N and water (i.e., Deltaproteobacteria). Further, resource additions elicited responses from 37% of bacterial species with species specializing on a specific resource (e.g., Chloroflexi) or being a generalist (e.g., Planctomycetes and Gammaproteobacteria). Our results offer the first direct links between legacy and priming effects on bacterial community composition and demonstrate that these mechanisms are not always complimentary leading to the formation of similar communities but may both be essential to maintain the high levels of bacterial diversity. Further, all resources produced elicited responders that were either specialists of generalists demonstrating that even bacteria in the extreme environment of Antarctica respond to pulses of resources.
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Le rôle des bactéries dans le filtrage du chlorométhane un gaz destructeur de la couche d'ozone : des souches modèles aux communautés microbiennes de sols forestiers / Bacteria as chloromethane sinks : from model strains to forest soil communitiesChaignaud, Pauline 29 June 2016 (has links)
Le chlorométhane (CH3Cl) est un composé organique volatile responsable de plus de 15 % de la dégradation de l’ozone stratosphérique due aux composés chlorés. Il est produit majoritairement par les plantes vivantes ou en décomposition. Les bactéries capables d’utiliser le CH3Cl comme source de carbone pour leur croissance peuvent jouer un rôle de filtre dans les émissions de CH3Cl vers l'atmosphère. Ce processus biologique reste à quantifier dans l'environnement, notamment pour les sols forestiers considérés comme un puits majeur de ce composé.Dans les études environnementales, le gène cmu A est utilisé comme biomarqueur de la dégradation bactérienne du CH3Cl. Il code une chlorométhane méthyltransférase essentielle à la croissance bactérienne avec le CH3Cl parla voie cmu (pour chloromethane utilisation), la seule caractérisée à ce jour. Mon projet de thèse avait un double objectif : i) l’approfondissement des connaissances de l’adaptation au CH3Cl chez une bactérie méthylotrophe modèle, Methylobacterium extorquens CM4; ii) l’exploration de la diversité des bactéries CH3Cl-dégradantes de sols forestiers. L’étude RNAseq chez la souche CM4 a montré que la croissance avec le CH3Cl s'accompagne de différences dans la transcription de 137 gènes de son génome (6.2 Mb) par rapport à sa croissance sur le méthanol (CH3OH). Les gènes de la voie cmu, ainsi que d’autres gènes impliqués dans le métabolisme de cofacteurs essentiels à l’utilisation du CH3Cl par cette voie et eux aussi portés par le plasmide pCMU01 de la souche, en font partie. Les paralogues de ces gènes localisés sur le chromosome ne sont quant à eux pas différentiellement exprimés. En revanche, d’autres gènes du chromosome, potentiellement impliqués dans l’excrétion de protons produits lors de la déshalogénation (hppA), la régénération du NADP+ (pnt), ou le métabolisme du cofacteur tétrahydrofolate(gènes gcvPHT), le sont. L’étude de la diversité des bactéries CH3Cl-dégradantes de sol forestier de la réserve naturelle de Steigerwald (Allemagne) a été réalisée sur des microcosmes par une approche de « Stable Isotope Probing ». Les microorganismes capables d’assimiler le CH3Cl marqué au [13C] incorporent cet isotope lourd du carbone dans leur ADN. L'analyse des séquences amplifiées par PCR des gènes codant l’ARN 16S des fractions d'ADN enrichies en [13C] a permis de mettre en évidence de nouveaux phylotypes, du genre Methylovirgula et de l’ordre des Actinomycetales, distincts de ceux auxquelles les souches dégradant le CH3Cl isolées jusqu'ici sont affiliées. En revanche, les séquences du gène cmuA et d’autres gènes du métabolisme méthylotrophe obtenues par PCR à partir de l'ADN enrichi en [13C] sont très proches de celles des souches CH3Cl-dégradantes connues. Les résultats obtenus suggèrent ainsi que des bactéries ayant acquis par transfert horizontal les gènes de dégradation de la voie cmu ou ne possédant pas de gène cmuA contribuent au filtrage biologique du CH3Cl des sols forestiers. A l'avenir, le couplage de différentes méthodes moléculaires et des approches culturales visera à découvrir de nouvelles voies microbiennes de l’utilisation du CH3Cl, et à caractériser l’abondance et la diversité des métabolismes impliqués dans la dégradation du CH3Cl dans les sols et d'autres compartiments environnementaux. / Chloromethane (CH3Cl) is a volatile organic compound responsible for over 15% of stratospheric ozone degradation due to chlorinated compounds. It is mainly produced by living and decaying plants. Bacteria utilizing CH3Cl as sole carbon and energy source for growth were shown to be involved in the filtering of CH3Cl emissions to the atmosphere. This biological process remains to be quantified in the environment, especially for forest soil, a major CH3Cl sink. The cmuA gene is used as a biomarker of bacterial CH3Cl degradation in environmental studies. It encodes a CH3Cl methyltransferase essential for bacterial growth by the cmu (chloromethane utilization) pathway for growth with CH3Cl and the only one characterized so far. My thesis project had a double aim: i) In depth studies of CH3Cl adaptation of a model methylotrophic bacterium, Methylobacterium extorquens strain CM4; ii) Exploration of bacterial CH3Cl-utilizers in forest. An RNAseq study of strain CM4 has shown that growth with CH3Cl leads to a difference of transcription of 137 genes in its 6.2 Mb genome compared to growth with methanol (CH3OH). Among those, genes of the cmu pathway and other genes involved in the metabolism of essential cofactors for CH3Cl utilization by this pathway, are all plasmid pCMU01-encoded. Paralogous genes located on the chromosome were not differentially expressed. On the other hand, other chromosomal genes potentially involved in extruding protons generated during CH3Cl deshalogenation (hppA), NADP+ regeneration (pnt), or in the cofactor tetrahydrofolate metabolism (gcvPHT) were differentially expressed. The diversity of CH3Cl-degrading bacteria in forest soil of the German natural park of Steigerwald was studied in microcosms using stable isotope probing. Microorganisms able to assimilate labeled [13C]- CH3Cl incorporate this heavy carbon isotope in their DNA. Sequence analysis of the PCR-amplified 16S RNA encoding gene from [13C]-DNA fractions uncovered phylotypes of the genus Methylovirgula and of the order of the Actinomycetales, which were not associated with bacterial CH3Cl degradation so far. In contrast, PCR-amplified sequences of cmuA and other genes of methylotrophic metabolism were closely related to known CH3Cl-degrading isolates. These results suggest that bacteria containing genes of the cmu pathway acquired by horizontal gene transfer as well as bacteria lacking the cmu pathway contribute to biological filtering of CH3Cl in forest soil. Future experiments coupling molecular and culture methods will aim to discover new CH3Cl-degrading pathways and to characterize the abundance and diversity of CH3Cl-degradation metabolism in soil and other environmental compartments.
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Descrição da comunidade microbiana associada à rizosfera de cana-de-açúcar / Description of Microbial Community in the Rhizosphere of SugarcaneDiogo Paes da Costa 24 January 2013 (has links)
A cana-de-açúcar é uma cultura importante no contexto agrário brasileiro, sobretudo com relação a manutenção e sustentabilidade dos agroecossistemas e da biodiversidade do solo. As comunidades microbianas associadas à canade- açúcar são participantes da manutenção dos ciclos biogeoquímicos, podendo ter sua estrutura e diversidade alteradas por mudanças no manejo da cultura e nas condições climáticas. Esse estudo teve como objetivo avaliar a diversidade microbiana associada à rizosfera de diferentes genótipos de cana-de-açúcar e empregar a metodologia de Stable Isotope Probing (DNA-SIP) para se avaliar a estrutura dos grupos responsivos a este ambiente. Para tanto, variedades de cana-de-açúcar foram selecionadas, extraindo-se o DNA total rizosférico e do bulk soil para análise por PCR-DGGE das regiões do gene 16S rDNA de bactérias, selecionando-se amostras representativas para o sequenciamento da região V6 do gene 16S rDNA através da plataforma Ion Torrent(TM). Os resultados demonstraram diferenças entre a diversidade das comunidades microbianas da rizosfera e do bulk soil, havendo a predominância dos grupos Actinobacteria, Proteobacteria e Acidobateria. Para o estudo da estrutura dos grupos responsivos na rizosfera, plantas da variedade RB86-7515 foram cultivadas sob duas concentrações de CO2 (350 e 700 ppm), realizando-se o enriquecimento com 13CO2, e posteriormente realizando a extração do DNA rizosférico para aplicação na técnica de DNA-SIP. A eficiência desta técnica foi avaliada por meio da técnica de PCR-DGGE para as regiões 16S rDNA de bactérias e ITS de fungos, onde foi verificado que após 48 horas já ocorre a incorporação de 13C pelas comunidades microbianas, havendo diferença entre os grupos que incorporaram o 13C. Diferenças foram também observadas para as distintas concentrações de CO2, indicando o DNA-SIP como uma poderosa ferramenta de estudos da ecologia das comunidades microbianas na rizosfera de cana-deaçúcar. / The sugarcane is an important crop in Brazilian agrarian context, especially in respect to maintenance and sustainability of agroecosystems and soil biodiversity. The microbial communities associated to sugarcane are involved biogeochemical cycles processes and it may have their structure and diversity changed due to crop management and climatic conditions. The aim of this study was to evaluate the microbial diversity associated to the rhizosphere of different sugarcane\'s genotypes and employ the Stable Isotope Probing tecnique (DNASIP) to evaluate the structure of the groups that are responding to this environment attributes. Therefore, some sugarcane varieties were selected and the total DNA in bulksoil and rhizosphere for analysis by PCR-DGGE of 16S rDNA gene regions of bacteria was extracted, selecting representative samples for sequencing the 16S rDNA gene of V6 region by Ion Torrent (TM) platform. The results showed differences between the diversity of microbial communities in the rhizosphere and bulk soil, with the predominance of Actinobacteria, Proteobacteria and Acidobateria groups. To study the structure of the responsive rhizosphere groups, the genotype RB86-7515 were grown under two CO2 concentrations (350 and 700 ppm), performing the 13CO2 enrichment. Afterwards, was performed the extraction of DNA for application of the SIP-rhizosphere DNA technique. The efficiency of this technique was assessed by PCR-DGGE over the regions of bacteria 16S rDNA and fungi ITS, which of these showed that occurs after 48 hours the incorporation of 13C by microbial communities, and it elucidate differences between the groups that incorporate the 13C. These differences were also observed for those different CO2 concentrations, indicating that the DNA-SIP is a powerful tool for studies of the ecology of microbial communities in the rhizosphere of sugarcane.
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