ABSTRACT
BACKGROUND: The systems-scale analysis of cellular metabolites, "metabolomics," provides data ideal for applications in metabolic engineering. However, many of the computational tools for strain design are built around Flux Balance Analysis (FBA), which makes assumptions that preclude direct integration of metabolomics data into the underlying models. Finding a way to retain the advantages of FBA's linear structure while relaxing some of its assumptions could allow us to account for metabolite levels and metabolite-dependent regulation in strain design tools built from FBA, improving the accuracy of predictions made by these tools. We designed, implemented, and characterized a modeling strategy based on Dynamic FBA (DFBA), called Linear Kinetics-Dynamic Flux Balance Analysis (LK-DFBA), to satisfy these specifications. Our strategy adds constraints describing the dynamics and regulation of metabolism that are strictly linear. We evaluated LK-DFBA against alternative modeling frameworks using simulated noisy data from a small in silico model and a larger model of central carbon metabolism in E. coli, and compared each framework's ability to recapitulate the original system. RESULTS: In the smaller model, we found that we could use regression from a dynamic flux estimation (DFE) with an optional non-linear parameter optimization to reproduce metabolite concentration dynamic trends more effectively than an ordinary differential equation model with generalized mass action rate laws when tested under realistic data sampling frequency and noise levels. We observed detrimental effects across all tested modeling approaches when metabolite time course data were missing, but found these effects to be smaller for LK-DFBA in most cases. With the E. coli model, we produced qualitatively reasonable results with similar properties to the smaller model and explored two different parameterization structures that yield trade-offs in computation time and accuracy. CONCLUSIONS: LK-DFBA allows for calculation of metabolite concentrations and considers metabolite-dependent regulation while still retaining many computational advantages of FBA. This provides the proof-of-principle for a new metabolic modeling framework with the potential to create genome-scale dynamic models and the potential to be applied in strain engineering tools that currently use FBA.
Subject(s)
Models, Biological , Escherichia coli/metabolism , Kinetics , MetabolomicsABSTRACT
BACKGROUND: Ruminants play a great role in sustainable livestock since they transform pastures, silage, and crop residues into high-quality human food (i.e. milk and beef). Animals with better ability to convert food into animal protein, measured as a trait called feed efficiency (FE), also produce less manure and greenhouse gas per kilogram of produced meat. Thus, the identification of high feed efficiency cattle is important for sustainable nutritional management. Our aim was to evaluate the potential of serum metabolites to identify FE of beef cattle before they enter the feedlot. RESULTS: A total of 3598 and 4210 m/z features was detected in negative and positive ionization modes via liquid chromatography-mass spectrometry. A single feature was different between high and low FE groups. Network analysis (WGCNA) yielded the detection of 19 and 20 network modules of highly correlated features in negative and positive mode respectively, and 1 module of each acquisition mode was associated with RFI (r = 0.55, P < 0.05). Pathway enrichment analysis (Mummichog) yielded the Retinol metabolism pathway associated with feed efficiency in beef cattle in our conditions. CONCLUSION: Altogether, these findings demonstrate the existence of a serum-based metabolomic signature associated with feed efficiency in beef cattle before they enter the feedlot. We are now working to validate the use of metabolites for identification of feed efficient animals for sustainable nutritional management.
Subject(s)
Animal Feed , Eating/genetics , Metabolome/genetics , Metabolomics/methods , Animal Nutritional Physiological Phenomena/genetics , Animals , Cattle , Eating/physiology , Food Quality , Phenotype , Red MeatABSTRACT
As genome-scale metabolic models become more sophisticated and dynamic, one significant challenge in using these models is to effectively integrate increasingly prevalent systems-scale metabolite profiling data into them. One common data processing step when integrating metabolite data is to smooth experimental time course measurements: the smoothed profiles can be used to estimate metabolite accumulation (derivatives), and thus the flux distribution of the metabolic model. However, this smoothing step is susceptible to the (often significant) noise in experimental measurements, limiting the accuracy of downstream model predictions. Here, we present several improvements to current approaches for smoothing metabolite time course data using defined functions. First, we use a biologically-inspired mathematical model function taken from transcriptional profiling and clustering literature that captures the dynamics of many biologically relevant transient processes. We demonstrate that it is competitive with, and often superior to, previously described fitting schemas, and may serve as an effective single option for data smoothing in metabolic flux applications. We also implement a resampling-based approach to buffer out sensitivity to specific data sets and allow for more accurate fitting of noisy data. We found that this method, as well as the addition of parameter space constraints, yielded improved estimates of concentrations and derivatives (fluxes) in previously described fitting functions. These methods have the potential to improve the accuracy of existing and future dynamic metabolic models by allowing for the more effective integration of metabolite profiling data.
Subject(s)
Metabolome , Metabolomics , Models, Biological , Algorithms , Escherichia coli/metabolism , Metabolomics/methods , Saccharomyces cerevisiae/metabolismABSTRACT
The goals of metabolic engineering are well-served by the biological information provided by metabolomics: information on how the cell is currently using its biochemical resources is perhaps one of the best ways to inform strategies to engineer a cell to produce a target compound. Using the analysis of extracellular or intracellular levels of the target compound (or a few closely related molecules) to drive metabolic engineering is quite common. However, there is surprisingly little systematic use of metabolomics datasets, which simultaneously measure hundreds of metabolites rather than just a few, for that same purpose. Here, we review the most common systematic approaches to integrating metabolite data with metabolic engineering, with emphasis on existing efforts to use whole-metabolome datasets. We then review some of the most common approaches for computational modeling of cell-wide metabolism, including constraint-based models, and discuss current computational approaches that explicitly use metabolomics data. We conclude with discussion of the broader potential of computational approaches that systematically use metabolomics data to drive metabolic engineering.
