Mapping Condition-Dependent Regulation of Lipid Metabolism in<i>Saccharomyces cerevisiae</i>

Jewett, Michael C.; Workman, Christopher T.; Nookaew, Intawat; Pizarro, Francisco; Agosín, Eduardo; Hellgren, Lars; Nielsen, Jens

doi:10.1534/g3.113.006601

Cited by 20 publications

(27 citation statements)

References 80 publications

(103 reference statements)

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“…Experimental measurements for the specific growth rate, specific substrate consumption rate and specific product formation rate in chemostat cultures under four different conditions were taken from our previous study [20] and compared to simulated data using FBA (for more information, see materials and methods and Additional file 5). The four conditions that were considered were carbon limited aerobic growth, nitrogen limited aerobic growth, carbon limited anaerobic growth and nitrogen limited anaerobic growth.…”

Section: Resultsmentioning

confidence: 99%

“…Chemostat cultivations were performed at a dilution rate of 0.05 h -1 under the same four different conditions as used for simulations above (carbon limited, nitrogen limited, aerobic and anaerobic) and microarray data as well as external and intracellular flux measurements was obtained for each condition [20]. We were particularly interested in changes that occur both on the transcript level and on the flux level, i.e.…”

Section: Resultsmentioning

confidence: 99%

“…Experimental data were collected from literature for chemostat cultivations performed at various dilution rates under each of the four different conditions: carbon limited aerobic [20,32-35], carbon limited anaerobic [36,37], nitrogen limited aerobic [35,36,38,39] and nitrogen limited anaerobic [40,41] (Additional file 5). For simulation purposes the uptake of glucose, NH 3 and oxygen were constrained in the model according to the measured values for each experiment.…”

Section: Methodsmentioning

confidence: 99%

“…Experimental data from chemostat cultivations from four different conditions (carbon limited, nitrogen limited, aerobic and anaerobic) was taken from Jewett et al [20]. The raw transcriptome data were normalized using the Probe Logarithmic Intensity Error (PLIER) method and the moderated t-statistic was used to identify significantly changed genes between two conditions.…”

Section: Methodsmentioning

confidence: 99%

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Mapping condition-dependent regulation of metabolism in yeast through genome-scale modeling

et al. 2013

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BackgroundThe genome-scale metabolic model of Saccharomyces cerevisiae, first presented in 2003, was the first genome-scale network reconstruction for a eukaryotic organism. Since then continuous efforts have been made in order to improve and expand the yeast metabolic network.ResultsHere we present iTO977, a comprehensive genome-scale metabolic model that contains more reactions, metabolites and genes than previous models. The model was constructed based on two earlier reconstructions, namely iIN800 and the consensus network, and then improved and expanded using gap-filling methods and by introducing new reactions and pathways based on studies of the literature and databases. The model was shown to perform well both for growth simulations in different media and gene essentiality analysis for single and double knock-outs. Further, the model was used as a scaffold for integrating transcriptomics, and flux data from four different conditions in order to identify transcriptionally controlled reactions, i.e. reactions that change both in flux and transcription between the compared conditions.ConclusionWe present a new yeast model that represents a comprehensive up-to-date collection of knowledge on yeast metabolism. The model was used for simulating the yeast metabolism under four different growth conditions and experimental data from these four conditions was integrated to the model. The model together with experimental data is a useful tool to identify condition-dependent changes of metabolism between different environmental conditions.

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Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

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Mapping condition-dependent regulation of metabolism in yeast through genome-scale modeling

et al. 2013

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“…The most typical approach is to use extracellular measurements (generally under chemostat conditions) to infer exchange fluxes used for FBA simulation, either as sole data 20,145,146 and as input in kinetic modeling [113][114][115]133,134 and other of the already reviewed methods 80,94,107,108,110,111,132,144 . The most typical approach is to use extracellular measurements (generally under chemostat conditions) to infer exchange fluxes used for FBA simulation, either as sole data 20,145,146 and as input in kinetic modeling [113][114][115]133,134 and other of the already reviewed methods 80,94,107,108,110,111,132,144 .…”

Section: 6metabolomicsmentioning

confidence: 99%

Genome scale models of yeast: towards standardized evaluation and consistent omic integration

Sánchez

Nielsen

2015

Integr. Biol.

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Genome scale models (GEMs) have enabled remarkable advances in systems biology, acting as functional databases of metabolism, and as scaffolds for the contextualization of high-throughput data. In the case of Saccharomyces cerevisiae (budding yeast), several GEMs have been published and are currently used for metabolic engineering and elucidating biological interactions. Here we review the history of yeast's GEMs, focusing on recent developments. We study how these models are typically evaluated, using both descriptive and predictive metrics. Additionally, we analyze the different ways in which all levels of omics data (from gene expression to flux) have been integrated in yeast GEMs. Relevant conclusions and current challenges for both GEM evaluation and omic integration are highlighted.

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Construction of mini‐chemostats for high‐throughput strain characterization

Bergenholm

Liu

Hansson

et al. 2019

Biotech & Bioengineering

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To achieve large‐scale, high‐throughput experiments for systems biology research of microorganisms, reliable data from robust cultivation systems are needed. Chemostats are such systems, ensuring reproducibility and quality by providing a stable, well‐controlled environment for the cells. However, many of the available chemostat systems require large amounts of media and are complex to set up and expensive to purchase and maintain. To address these concerns, we developed a mini‐chemostat (MC) system with 16 reactors, each at a working volume of 40 ml. Sensors measure dissolved oxygen in the reactor, while OD600 is measured in the outflow. We further developed a CO2 and pH sensor array that can be plugged into the outflow of the reactors. The system was used to characterize yeast physiology at four metabolically different conditions: limitations of glucose, both aerobic and anaerobic, nitrogen, and ethanol. The physiology of yeast cells grown at the four different conditions in the MC system was compared with the yeast cells grown in a DASGIP 1 L system using RNAseq analysis. The results show that the MC system provides the same environmental conditions as the DASGIP system and that the MC system is reproducible between different runs. The system is built to be easily scalable with more reactors and to include more sensors, if available. Our study shows that a robust, reproducible chemostat system for high‐throughput and large‐scale experiments can be built at low costs.

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Mapping Condition-Dependent Regulation of Lipid Metabolism inSaccharomyces cerevisiae

Cited by 20 publications

References 80 publications

Mapping condition-dependent regulation of metabolism in yeast through genome-scale modeling

Mapping condition-dependent regulation of metabolism in yeast through genome-scale modeling

Genome scale models of yeast: towards standardized evaluation and consistent omic integration

Construction of mini‐chemostats for high‐throughput strain characterization

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