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BACKGROUND: Antimicrobial resistance is a major global health challenge. Metagenomics allows analyzing the presence and dynamics of "resistomes" (the ensemble of genes encoding antimicrobial resistance in a given microbiome) in disparate microbial ecosystems. However, the low sensitivity and specificity of available metagenomic methods preclude the detection of minority populations (often present below their detection threshold) and/or the identification of allelic variants that differ in the resulting phenotype. Here, we describe a novel strategy that combines targeted metagenomics using last generation in-solution capture platforms, with novel bioinformatics tools to establish a standardized framework that allows both quantitative and qualitative analyses of resistomes. METHODS: We developed ResCap, a targeted sequence capture platform based on SeqCapEZ (NimbleGene) technology, which includes probes for 8667 canonical resistance genes (7963 antibiotic resistance genes and 704 genes conferring resistance to metals or biocides), and 2517 relaxase genes (plasmid markers) and 78,600 genes homologous to the previous identified targets (47,806 for antibiotics and 30,794 for biocides or metals). Its performance was compared with metagenomic shotgun sequencing (MSS) for 17 fecal samples (9 humans, 8 swine). ResCap significantly improves MSS to detect "gene abundance" (from 2.0 to 83.2%) and "gene diversity" (26 versus 14.9 genes unequivocally detected per sample per million of reads; the number of reads unequivocally mapped increasing up to 300-fold by using ResCap), which were calculated using novel bioinformatic tools. ResCap also facilitated the analysis of novel genes potentially involved in the resistance to antibiotics, metals, biocides, or any combination thereof. CONCLUSIONS: ResCap, the first targeted sequence capture, specifically developed to analyze resistomes, greatly enhances the sensitivity and specificity of available metagenomic methods and offers the possibility to analyze genes related to the selection and transfer of antimicrobial resistance (biocides, heavy metals, plasmids). The model opens the possibility to study other complex microbial systems in which minority populations play a relevant role. ; This study was supported by the European Commission, Seven Framework Program (EVOTARFP7-HEALTH-282004 for VFL, FB, JLM, AA, DE, ER, RJLW, WvS, FdlC, and TMC), the Joint Programming Initiative in Antimicrobial Resistance (JPIAMR Third call, STARCS, JPIAMR2016-AC16/00039 to TMC, RJLW, WvS), the Joint Programming Initiative in Water (JPI Water StARE JPIW2013-089-C02-01 to JLM) and the Ministry of Economy and Competitiveness of Spain (BIO2014-54507-R to JLM, and PLASWIRES-612146/FP7-ICT-2013-10 and BFU2014-55534-C2-1-P for FdlC). The authors also acknowledge the European Development Regional Fund "A way to achieve Europe" (ERDF) for co-founding the Spanish R&D National Plan 2012-2019 (BIO2014-54507-R to JLM, PI15-0512 to TMC, PI15-00818 to FB, and BFU2014-55534-C2-1-P to FdlC), CIBER (CIBER in Epidemiology and Public Health, CIBERESP; CB06/02/0053 to FB), the Spanish Network for Research on Infectious Diseases (REIPI RD12/0015 to JLM) and the Regional Government of Madrid (InGeMICSB2017/BMD-3691). Val F. Lanza was further funded by a Research Award Grant 2016 of the European Society for Clinical Microbiology and Infectious Diseases (ESCMID). Additional funding was from the Metagenopolis grant ANR-11-DPBS-0001 to DE.

[Background]: Antimicrobial resistance is a major global health challenge. Metagenomics allows analyzing the presence and dynamics of "resistomes" (the ensemble of genes encoding antimicrobial resistance in a given microbiome) in disparate microbial ecosystems. However, the low sensitivity and specificity of available metagenomic methods preclude the detection of minority populations (often present below their detection threshold) and/or the identification of allelic variants that differ in the resulting phenotype. Here, we describe a novel strategy that combines targeted metagenomics using last generation in-solution capture platforms, with novel bioinformatics tools to establish a standardized framework that allows both quantitative and qualitative analyses of resistomes. [Methods]: We developed ResCap, a targeted sequence capture platform based on SeqCapEZ (NimbleGene) technology, which includes probes for 8667 canonical resistance genes (7963 antibiotic resistance genes and 704 genes conferring resistance to metals or biocides), and 2517 relaxase genes (plasmid markers) and 78,600 genes homologous to the previous identified targets (47,806 for antibiotics and 30,794 for biocides or metals). Its performance was compared with metagenomic shotgun sequencing (MSS) for 17 fecal samples (9 humans, 8 swine). ResCap significantly improves MSS to detect "gene abundance" (from 2.0 to 83.2%) and "gene diversity" (26 versus 14.9 genes unequivocally detected per sample per million of reads; the number of reads unequivocally mapped increasing up to 300-fold by using ResCap), which were calculated using novel bioinformatic tools. ResCap also facilitated the analysis of novel genes potentially involved in the resistance to antibiotics, metals, biocides, or any combination thereof. [Conclusions]: ResCap, the first targeted sequence capture, specifically developed to analyze resistomes, greatly enhances the sensitivity and specificity of available metagenomic methods and offers the possibility to analyze genes related to the selection and transfer of antimicrobial resistance (biocides, heavy metals, plasmids). The model opens the possibility to study other complex microbial systems in which minority populations play a relevant role. ; This study was supported by the European Commission, Seven Framework Program (EVOTARFP7-HEALTH-282004 for VFL, FB, JLM, AA, DE, ER, RJLW, WvS, FdlC, and TMC), the Joint Programming Initiative in Antimicrobial Resistance (JPIAMR Third call, STARCS, JPIAMR2016-AC16/00039 to TMC, RJLW, WvS), the Joint Programming Initiative in Water (JPI Water StARE JPIW2013-089-C02-01 to JLM) and the Ministry of Economy and Competitiveness of Spain (BIO2014-54507-R to JLM, and PLASWIRES-612146/FP7-ICT-2013-10 and BFU2014-55534-C2-1-P for FdlC). The authors also acknowledge the European Development Regional Fund "A way to achieve Europe" (ERDF) for co-founding the Spanish R&D National Plan 2012-2019 (BIO2014-54507-R to JLM, PI15-0512 to TMC, PI15-00818 to FB, and BFU2014-55534-C2-1-P to FdlC), CIBER (CIBER in Epidemiology and Public Health, CIBERESP; CB06/02/0053 to FB), the Spanish Network for Research on Infectious Diseases (REIPI RD12/0015 to JLM) and the Regional Government of Madrid (InGeMICS- B2017/BMD-3691). Val F. Lanza was further funded by a Research Award Grant 2016 of the European Society for Clinical Microbiology and Infectious Diseases (ESCMID). Additional funding was from the Metagenopolis grant ANR-11-DPBS-0001 to DE. ; Peer reviewed

Technologies such as next generation sequencing (NGS) are transforming research fields at the methodological, conceptual, and organizational level. They open up new possibilities and bring with them new commitments and inherent limitations. We show from a philosophy of science perspective how NGS-based metagenomics has transformed microbial ecology and, with it, parts of agricultural soil science, which integrate ecological approaches with the aim to inform agricultural practices. We reconstruct agricultural science as design science (sensu Niiniluoto) and describe how the possibilities, commitments, and limitations of metagenomics approaches in microbial ecology shape values, situation assessments, and recommendations for interventions of soil microbiology in the context of sustainable agriculture.

Written by renowned researchers specialised in the most relevant and emerging topics in the field, this book provides comprehensive information on the new theoretical, methodological and applied aspects of metagenomics and other 'omics' approaches used to study the microbial N cycle. Recommended for microbiologists, environmental scientists and anyone interested in microbial communities, metagenomics, metatranscriptomics and metaproteomics of the microbial N cycle. This volume provides a thorough account of the contributions of metagenomics to microbial N cycle background theory, reviews state-of-the-art investigative methods and explores new applications in water treatment, agricultural practices and climate change, among others.

Targeted metagenomics is the study of the composition of microbial communities in diverse biological samples, based on the sequencing of a genomic locus. This application has boomed over the last decade thanks to the democratisation of high-throughput sequencing, and has allowed substantial progress in the study of microbial evolution and diversity. However, new problems have emerged with high-throughput sequencing : the exponential generation of data must be properly analyzed with bioinformatics tools fitted to the experimental designs and associated biological questions. This dissertation provides solutions to improve targeted metagenomics studies, by the development of new tools and methods allowing a better understanding of analytical biases, and a better design of experiments. Firstly, an expert assessment of the analytical pipeline used on the PEGASE-biosciences plateform has been performed. This assessment revealed the need of a formal evaluation method of analytical pipelines used for targeted metagenomics analyses. This method has been developed with simulated and real datasets, and adequate evaluation metrics. It has been used on several analytical pipelines commonly used by the scientific community, as well as on new analytical methods which have never been used in such a context before. This evaluation allowed to better understand experimental design biases, which can affect the results and biological conclusions. One of those major biases is the design of amplification primers to target the genomic locus of interest. A primer design software, adaptable to different experimental designs, has been specifically developed to minimize this bias. Finally, analytical guidelines and experimental design recommendations have been formulated to improve targeted metagenomics studies. ; La métagénomique ciblée, étude de la composition et de la diversité des communautés microbiennes présentes dans différents échantillon biologiques sur la base d'un marqueur génomique, a connu un véritable essor lors de cette ...

Targeted metagenomics is the study of the composition of microbial communities in diverse biological samples, based on the sequencing of a genomic locus. This application has boomed over the last decade thanks to the democratisation of high-throughput sequencing, and has allowed substantial progress in the study of microbial evolution and diversity. However, new problems have emerged with high-throughput sequencing : the exponential generation of data must be properly analyzed with bioinformatics tools fitted to the experimental designs and associated biological questions. This dissertation provides solutions to improve targeted metagenomics studies, by the development of new tools and methods allowing a better understanding of analytical biases, and a better design of experiments. Firstly, an expert assessment of the analytical pipeline used on the PEGASE-biosciences plateform has been performed. This assessment revealed the need of a formal evaluation method of analytical pipelines used for targeted metagenomics analyses. This method has been developed with simulated and real datasets, and adequate evaluation metrics. It has been used on several analytical pipelines commonly used by the scientific community, as well as on new analytical methods which have never been used in such a context before. This evaluation allowed to better understand experimental design biases, which can affect the results and biological conclusions. One of those major biases is the design of amplification primers to target the genomic locus of interest. A primer design software, adaptable to different experimental designs, has been specifically developed to minimize this bias. Finally, analytical guidelines and experimental design recommendations have been formulated to improve targeted metagenomics studies. ; La métagénomique ciblée, étude de la composition et de la diversité des communautés microbiennes présentes dans différents échantillon biologiques sur la base d'un marqueur génomique, a connu un véritable essor lors de cette ...

Targeted metagenomics is the study of the composition of microbial communities in diverse biological samples, based on the sequencing of a genomic locus. This application has boomed over the last decade thanks to the democratisation of high-throughput sequencing, and has allowed substantial progress in the study of microbial evolution and diversity. However, new problems have emerged with high-throughput sequencing : the exponential generation of data must be properly analyzed with bioinformatics tools fitted to the experimental designs and associated biological questions. This dissertation provides solutions to improve targeted metagenomics studies, by the development of new tools and methods allowing a better understanding of analytical biases, and a better design of experiments. Firstly, an expert assessment of the analytical pipeline used on the PEGASE-biosciences plateform has been performed. This assessment revealed the need of a formal evaluation method of analytical pipelines used for targeted metagenomics analyses. This method has been developed with simulated and real datasets, and adequate evaluation metrics. It has been used on several analytical pipelines commonly used by the scientific community, as well as on new analytical methods which have never been used in such a context before. This evaluation allowed to better understand experimental design biases, which can affect the results and biological conclusions. One of those major biases is the design of amplification primers to target the genomic locus of interest. A primer design software, adaptable to different experimental designs, has been specifically developed to minimize this bias. Finally, analytical guidelines and experimental design recommendations have been formulated to improve targeted metagenomics studies. ; La métagénomique ciblée, étude de la composition et de la diversité des communautés microbiennes présentes dans différents échantillon biologiques sur la base d'un marqueur génomique, a connu un véritable essor lors de cette dernière décennie grâce à l'arrivée du séquençage haut-débit. Faisant appel à des outils de biologie moléculaire et de bioinformatique, elle a été à l'origine de substantiels progrès dans les domaines de l'évolution et de la diversité microbienne. Cependant, de nouvelles problématiques sont apparues avec le séquençage haut-débit : la génération exponentielle de données soulève des problèmes d'analyse bioinformatique, qui doit être adaptée aux plans d'expérience et aux questions biologiques associées. Cette thèse propose des solutions d'amélioration des études de métagénomique ciblée par le développement d'outils et de méthodes innovantes, apportant une meilleure compréhension des biais d'analyse inhérents à de telles études, et une meilleure conception des plans d'expérience. Tout d'abord, une expertise du pipeline d'analyse utilisé en production sur la plate-forme PEGASE-biosciences a été menée. Cette évaluation a révélé la nécessité de mettre en place une méthode d'évaluation formelle de pipelines d'analyses de données de métagénomique ciblée, qui a été développée sur la base de données simulées et réelles, et de métriques d'évaluation adaptées. Cette méthode a été utilisée sur plusieurs pipelines d'analyse couramment utilisés par la communauté, tout comme sur de nouvelles approches d'analyse jamais utilisées dans un tel contexte. Cette évaluation a permis de mieux comprendre les biais du plan d'expérience qui peuvent affecter les résultats et les conclusions biologiques associées. Un de ces biais majeurs est le choix des amorces d'amplification de la cible ; un logiciel de design d'amorces adaptées au plan d'expérience a été spécifiquement développé pour minimiser ce biais. Enfin, des recommandations de montage de plan d'expérience et d'analyse ont été émises afin d'améliorer la robustesse des études de métagénomique ciblée.

Targeted metagenomics is the study of the composition of microbial communities in diverse biological samples, based on the sequencing of a genomic locus. This application has boomed over the last decade thanks to the democratisation of high-throughput sequencing, and has allowed substantial progress in the study of microbial evolution and diversity. However, new problems have emerged with high-throughput sequencing : the exponential generation of data must be properly analyzed with bioinformatics tools fitted to the experimental designs and associated biological questions. This dissertation provides solutions to improve targeted metagenomics studies, by the development of new tools and methods allowing a better understanding of analytical biases, and a better design of experiments. Firstly, an expert assessment of the analytical pipeline used on the PEGASE-biosciences plateform has been performed. This assessment revealed the need of a formal evaluation method of analytical pipelines used for targeted metagenomics analyses. This method has been developed with simulated and real datasets, and adequate evaluation metrics. It has been used on several analytical pipelines commonly used by the scientific community, as well as on new analytical methods which have never been used in such a context before. This evaluation allowed to better understand experimental design biases, which can affect the results and biological conclusions. One of those major biases is the design of amplification primers to target the genomic locus of interest. A primer design software, adaptable to different experimental designs, has been specifically developed to minimize this bias. Finally, analytical guidelines and experimental design recommendations have been formulated to improve targeted metagenomics studies. ; La métagénomique ciblée, étude de la composition et de la diversité des communautés microbiennes présentes dans différents échantillon biologiques sur la base d'un marqueur génomique, a connu un véritable essor lors de cette dernière décennie grâce à l'arrivée du séquençage haut-débit. Faisant appel à des outils de biologie moléculaire et de bioinformatique, elle a été à l'origine de substantiels progrès dans les domaines de l'évolution et de la diversité microbienne. Cependant, de nouvelles problématiques sont apparues avec le séquençage haut-débit : la génération exponentielle de données soulève des problèmes d'analyse bioinformatique, qui doit être adaptée aux plans d'expérience et aux questions biologiques associées. Cette thèse propose des solutions d'amélioration des études de métagénomique ciblée par le développement d'outils et de méthodes innovantes, apportant une meilleure compréhension des biais d'analyse inhérents à de telles études, et une meilleure conception des plans d'expérience. Tout d'abord, une expertise du pipeline d'analyse utilisé en production sur la plate-forme PEGASE-biosciences a été menée. Cette évaluation a révélé la nécessité de mettre en place une méthode d'évaluation formelle de pipelines d'analyses de données de métagénomique ciblée, qui a été développée sur la base de données simulées et réelles, et de métriques d'évaluation adaptées. Cette méthode a été utilisée sur plusieurs pipelines d'analyse couramment utilisés par la communauté, tout comme sur de nouvelles approches d'analyse jamais utilisées dans un tel contexte. Cette évaluation a permis de mieux comprendre les biais du plan d'expérience qui peuvent affecter les résultats et les conclusions biologiques associées. Un de ces biais majeurs est le choix des amorces d'amplification de la cible ; un logiciel de design d'amorces adaptées au plan d'expérience a été spécifiquement développé pour minimiser ce biais. Enfin, des recommandations de montage de plan d'expérience et d'analyse ont été émises afin d'améliorer la robustesse des études de métagénomique ciblée.

Targeted metagenomics is the study of the composition of microbial communities in diverse biological samples, based on the sequencing of a genomic locus. This application has boomed over the last decade thanks to the democratisation of high-throughput sequencing, and has allowed substantial progress in the study of microbial evolution and diversity. However, new problems have emerged with high-throughput sequencing : the exponential generation of data must be properly analyzed with bioinformatics tools fitted to the experimental designs and associated biological questions. This dissertation provides solutions to improve targeted metagenomics studies, by the development of new tools and methods allowing a better understanding of analytical biases, and a better design of experiments. Firstly, an expert assessment of the analytical pipeline used on the PEGASE-biosciences plateform has been performed. This assessment revealed the need of a formal evaluation method of analytical pipelines used for targeted metagenomics analyses. This method has been developed with simulated and real datasets, and adequate evaluation metrics. It has been used on several analytical pipelines commonly used by the scientific community, as well as on new analytical methods which have never been used in such a context before. This evaluation allowed to better understand experimental design biases, which can affect the results and biological conclusions. One of those major biases is the design of amplification primers to target the genomic locus of interest. A primer design software, adaptable to different experimental designs, has been specifically developed to minimize this bias. Finally, analytical guidelines and experimental design recommendations have been formulated to improve targeted metagenomics studies. ; La métagénomique ciblée, étude de la composition et de la diversité des communautés microbiennes présentes dans différents échantillon biologiques sur la base d'un marqueur génomique, a connu un véritable essor lors de cette dernière décennie grâce à l'arrivée du séquençage haut-débit. Faisant appel à des outils de biologie moléculaire et de bioinformatique, elle a été à l'origine de substantiels progrès dans les domaines de l'évolution et de la diversité microbienne. Cependant, de nouvelles problématiques sont apparues avec le séquençage haut-débit : la génération exponentielle de données soulève des problèmes d'analyse bioinformatique, qui doit être adaptée aux plans d'expérience et aux questions biologiques associées. Cette thèse propose des solutions d'amélioration des études de métagénomique ciblée par le développement d'outils et de méthodes innovantes, apportant une meilleure compréhension des biais d'analyse inhérents à de telles études, et une meilleure conception des plans d'expérience. Tout d'abord, une expertise du pipeline d'analyse utilisé en production sur la plate-forme PEGASE-biosciences a été menée. Cette évaluation a révélé la nécessité de mettre en place une méthode d'évaluation formelle de pipelines d'analyses de données de métagénomique ciblée, qui a été développée sur la base de données simulées et réelles, et de métriques d'évaluation adaptées. Cette méthode a été utilisée sur plusieurs pipelines d'analyse couramment utilisés par la communauté, tout comme sur de nouvelles approches d'analyse jamais utilisées dans un tel contexte. Cette évaluation a permis de mieux comprendre les biais du plan d'expérience qui peuvent affecter les résultats et les conclusions biologiques associées. Un de ces biais majeurs est le choix des amorces d'amplification de la cible ; un logiciel de design d'amorces adaptées au plan d'expérience a été spécifiquement développé pour minimiser ce biais. Enfin, des recommandations de montage de plan d'expérience et d'analyse ont été émises afin d'améliorer la robustesse des études de métagénomique ciblée.

The shortage of wild fishery resources and the rising demand for human nutrition has driven a great expansion in aquaculture during the last decades in terms of production and economic value. As such, sustainable aquaculture production is one of the main priorities of the European Union's 2030 agenda. However, the intensification of seafood farming has resulted in higher risks of disease outbreaks and in the increased use of antimicrobials to control them. The selective pressure exerted by these drugs provides the ideal conditions for the emergence of antimicrobial resistance hotspots in aquaculture facilities. Omics technology is an umbrella term for modern technologies such as genomics, metagenomics, transcriptomics, proteomics, culturomics, and metabolomics. These techniques have received increasing recognition because of their potential to unravel novel mechanisms in biological science. Metagenomics allows the study of genomes in microbial communities contained within a certain environment. The potential uses of metagenomics in aquaculture environments include the study of microbial diversity, microbial functions, and antibiotic resistance genes. A snapshot of these high throughput technologies applied to microbial diversity and antimicrobial resistance studies in aquacultures will be presented in this review. ; info:eu-repo/semantics/publishedVersion

Conservation strategies require multifaceted approaches to monitor and protect primate populations, many of which are rapidly declining around the world. We propose that microbial ecology and next-generation microbiome analyses offer valuable perspectives and tools for investigating and monitoring primate health and improving conservation efforts. The microbial communities inhabiting primates and other taxa profoundly affect host health, nutrition, physiology, and immune systems, through relationships that range from commensal and mutualistic to pathogenic. Recent advances in DNA sequencing now make it feasible and economically viable to identify microbiomes among and within hosts. Herein, we highlight several examples in which microbial analyses of primates can aid conservation approaches that are broadly applicable across other taxa. First, we highlight evidence for clear spatial variation (e.g. biogeographic niche specificity, both within the anatomical regions of the host body, as well as in the geographic location of the host) and temporal (e.g. seasonal, ontogenetic) patterns in microbial distribution. We emphasize that microbial communities are sensitive to alterations in the external environment and that microbial diversity correlates with habitat quality, imposing direct health consequences. Incorporating microbial host and biogeographic variation holds great potential for forest corridor assessments and for reintroduction efforts. Finally, microbial pathogens transmitted between humans and wild primate populations carry both direct and indirect conservation implications. Principally, we argue that phylogenetic analyses of infectious pathogens (e.g., Ebola, dengue, Borellia, and Treponema) can aid our understanding of modes of disease transmission and aid conservation disease abatement efforts. The application of microbial analyses to conservation is currently in its infancy but holds enormous potential. To date, no conservation policy or legislation includes microbiome assessments. Integrating new ...

Publisher's version (útgefin grein) ; Antimicrobial resistance (AMR) is a serious threat to global public health, but obtaining representative data on AMR for healthy human populations is difficult. Here, we use metagenomic analysis of untreated sewage to characterize the bacterial resistome from 79 sites in 60 countries. We find systematic differences in abundance and diversity of AMR genes between Europe/North-America/Oceania and Africa/Asia/South-America. Antimicrobial use data and bacterial taxonomy only explains a minor part of the AMR variation that we observe. We find no evidence for cross-selection between antimicrobial classes, or for effect of air travel between sites. However, AMR gene abundance strongly correlates with socio-economic, health and environmental factors, which we use to predict AMR gene abundances in all countries in the world. Our findings suggest that global AMR gene diversity and abundance vary by region, and that improving sanitation and health could potentially limit the global burden of AMR. We propose metagenomic analysis of sewage as an ethically acceptable and economically feasible approach for continuous global surveillance and prediction of AMR. ; We are grateful to Hanne Nørgaard Nielsen, Christina Aaby Svendsen, Jacob Dyring Jensen, Birthe S. Rosenqvist Lund, Kate Vina Vibefeldt, Inge Marianne Hansen, Gunhild Larsen, Hanne Mordhorst, and Carsten Bidstrup for technical assistance. We also thank Jeffrey Edward Skiby for internal review. This study has received funding from the European Union's Horizon 2020 research and innovation programme under grant agreement no. 643476 (COMPARE), the World Health Organization, The Villum Foundation (VKR023052), and The Novo Nordisk Foundation (NNF16OC0021856: Global Surveillance of Antimicrobial Resistance). ; Peer Reviewed

Little is known about the diversity and structuring of freshwater microbial communities beyond the patterns revealed by tracing their distribution in the landscape with common taxonomic markers such as the ribosomal RNA. To address this gap in knowledge, metagenomes from temperate lakes were compared to selected marine metagenomes. Taxonomic analyses of rRNA genes in these freshwater metagenomes confirm the previously reported dominance of a limited subset of uncultured lineages of freshwater bacteria, whereas Archaea were rare. Diversification into marine and freshwater microbial lineages was also reflected in phylogenies of functional genes, and there were also significant differences in functional beta-diversity. The pathways and functions that accounted for these differences are involved in osmoregulation, active transport, carbohydrate and amino acid metabolism. Moreover, predicted genes orthologous to active transporters and recalcitrant organic matter degradation were more common in microbial genomes from oligotrophic versus eutrophic lakes. This comparative metagenomic analysis allowed us to formulate a general hypothesis that oceanic- compared with freshwater-dwelling microorganisms, invest more in metabolism of amino acids and that strategies of carbohydrate metabolism differ significantly between marine and freshwater microbial communities. ; This work was supported by the Swedish Foundation for Strategic Research (Grant Number ICA10-0015 to AE), the Swedish Research Council (Grant Numbers 349-2007-831, 621-2008-3259 and 621-2011-4669 to SGEA; 2009-3784, 2008-1923 and 2012-3892 to SB), the National Science Foundation [Awards CBET-0644949 (CAREER), MCB-0702653 (Microbial Observatories Program) to KD and DEB-841933 to RS], DEB-0822700 (Long Term Ecological Research, NTL LTER to KDM), the European Union (grant to SGEA), the Göran Gustafsson Foundation (grant to SGEA), the Knut and Alice Wallenberg Foundation (Grant Numbers KAW-2011.0148 and KAW-2012.0075 to SGEA), and the Swedish Wennergren Foundation (to KDM and SB).